Antibodies and antigen-binding fragments that specifically bind to microtubule-associated protein tau

ABSTRACT

The disclosure relates to antibodies and antigen-binding fragments that specifically bind to microtubule-associated protein tau. The disclosure also relates to diagnostic, prophylactic and therapeutic methods using anti-tau antibodies.

CROSS REFERENCE TO RELATED APPLICATION

This application is a continuation of U.S. patent application Ser. No. 15/321,680, filed on Dec. 22, 2016, which is a national phase entry under 35 U.S.C. § 371 of International Patent Application PCT/EP2015/064529, filed Jun. 26, 2015, designating the United States of America and published in English as International Patent Publication WO 2015/197820 A1 on Dec. 30, 2015, which claims the benefit under Article 8 of the Patent Cooperation Treaty to European Patent Application Serial Nos. 14179699.5, 14179706.8, 14179719.1, and 14179739.9, all filed on Aug. 4, 2014, and to U.S. Provisional Patent Application Ser. Nos. 62/017,746, 62/017,789, 62/017,807, and 62/017,812, all filed on Jun. 26, 2014, the entire disclosure of which is hereby incorporated by reference for all purposes as if fully set forth herein.

STATEMENT ACCORDING To 37 C.F.R. § 1.821(C) OR (E)—SEQUENCE LISTING SUBMITTED AS ASCII TEXT FILE

Pursuant to 37 C.F.R. 1.821(c) or (e), a file containing an ASCII text version of the Sequence Listing has been submitted concomitant with this application, the contents of which are hereby incorporated by reference.

TECHNICAL FIELD

The application relates to medicine. The disclosure, in particular, relates to antibodies and antigen-binding fragments that specifically bind to microtubule-associated protein tau. The disclosure also relates to diagnostic, prophylactic and therapeutic methods using anti-tau antibodies.

BACKGROUND

Dementia is a syndrome that can be caused by a number of progressive disorders that affect memory, thinking, behavior and the ability to perform everyday activities. About 36 million people worldwide are suffering from dementia today. The number of people with dementia is projected to double by 2030, and more than triple to 115.4 million people by 2050. Alzheimer's disease (AD) is the most common type of dementia. Currently, one in nine people age 65 and older (11 percent) and nearly half of those over age 85 have Alzheimer's disease. According to Alzheimer's Disease International, current global costs of caring for these patients exceeds $600 billion annually. These costs are likely to rise even faster than the prevalence of disease, especially in the developing world, as more formal social care systems emerge, and rising incomes lead to higher opportunity costs (B. Winblad and L. Jonsson, World Alzheimer Report 2010).

The brains of AD patients have an abundance of two abnormal structures, amyloid plaques and neurofibrillary tangles. This is especially true in certain regions of the brain that are important in memory. There is also a substantial loss of neurons and synapses in the cerebral cortex and certain subcortical regions. Both neurofibrillary tangles and neuronal loss increase in parallel with the duration and severity of illness (T. Gomez-Isla et al., Ann. Neurol. 1997; 41:17-24) and neurofibrillary load has been shown to correlate with cognitive decline (H. Braak and E. Braak, Neurobiol. Aging 1997 July-August; 18(4):351-7).

Neurofibrillary tangles are intraneuronal lesions that are composed of hyperphosphorylated and insoluble accumulations of the microtubule-associated protein, tau. These accumulations are a histopathological feature of many neurodegenerative diseases, which are collectively known as tauopathies. Tauopathies include, e.g., Alzheimer's disease (AD), Pick's disease (PiD), progressive supranuclear palsy (PSP), corticobasal degeneration (CBD), and frontotemporal lobar degeneration (FTLD). In human tauopathies, pathology progresses from one brain region to another in disease-specific patterns (H. Braak and E. Braak, Neurobiol. Aging 1997 July-August; 18(4):351-7; Raj et al., Neuron. 2012; 73:1204-1215; Seeley et al., Neuron. 2009; 62:42-52; and Zhou et al. Neuron. 2012; 73:1216-1227), the underlying mechanism of which is not yet clear.

Tau pathology is involved in and may be a cause of many tauopathies. In its normal form, tau is a highly soluble microtubule-associated protein (Jeganathan et al., Biochemistry 2008, 47:10526-10539) that binds and promotes the assembly of microtubules (Drechsel et al., Mol. Biol. Cell. 1992, 3:1141-1154). However, in tauopathies, tau becomes hyperphosphorylated, causing detachment from microtubules, and ultimately accumulation as neurofibrillary tangles that are visualized within dystrophic neurites and cell bodies (Mandelkow and Mandelkow, Cold Spring Harbor, Perspect. Med. 2, 2012: a006247). The amount of tau pathology correlates with progressive neuronal dysfunction, synaptic loss, and functional decline in humans and transgenic mouse models (Arriagada et al., Neurology 1992 March; 42(3 Pt 1):631-9; Bancher et al., Neurosci. Lett. 1993, 162:179-182; Polydoro et al., J. Neuroscience 2009, 29:10741-10749; and Small and Duff, Neuron. 2008 Nov. 26; 60(4):534-42). While there have been no tau mutations observed in Alzheimer's disease, mutations in the tau gene appear to cause some forms of frontotemporal dementia (Cairns et al., Am. J. Pathol. 2007, 171:227-40), presenting with tau-positive inclusions and signifying that tau dysfunction is sufficient to cause neurodegeneration. Moreover, pathological tau appears to be an integral part of Aβ-induced neurotoxicity in cell culture and transgenic animal models (M. Rapoport, PNAS 2002, 99:9, 6364-6369; E. D. Roberson et al., Science 2007, 316:750-754; A. M. Nicholson and A. Ferreira, J. Neurosci. 2009, 29:4640-4651; H. Oakley, J. Neurosci. 2006, 26(40):10129-10140).

Passive and active immunizations against tau have been analyzed in mice using several different mouse models, including different phospho-tau peptides for active immunizations and anti-tau antibodies for passive immunotherapy (A. A. Asuni et al., J. Neurosci. 2007, 27(34):9115-9129; E. M. Sigurdsson, Curr. Alzheimer Res. 2009, 6(5):446-450; A. Boutajangout et al., J. Neurosci. 2010, 30(49):16559-16566; H. Rosenmann et al., Arch. Neurol. 2006, 63(10):1459-1467; M. Boimel et al., Exp. Neurol. 2010, 224(2):472-485). In the first report describing immunizations with a 30-amino acid phosphorylated tau peptide, an effect on the ratios of soluble and insoluble tau, reduction of tangle formation in the immunized mice, and functional benefits observed in behavior testing for these mice were shown (A. Boutajangout et al., J. Neuroscience 2010, 30:16559-16566). Passive immunization with well-characterized anti-tau antibodies, which react with phosphorylated Ser396 and Ser404 of the hyperphosphorylated tau protein at an early pathologic conformational epitope on tau, confirmed the results seen in active immunization studies. Mice treated with these antibodies showed marked reductions in tau pathology, which was measured by biochemical methods and histology, as well as a significant delay in loss of motor-function decline that was assessed in behavioral testing (A. Boutajangout et al., J. Neurochem. 2011, 118(4):658-667; X. Chai et al., J. Biol. Chem. 2011, 286(39):34457-34467).

Tau-based therapies have only been analyzed in mouse models to date. But in view of the severity of tauopathies in general, and to the cost to society of Alzheimer's disease specifically, there is an ongoing need for effective means to diagnose, monitor, prevent and treat tauopathies.

BRIEF SUMMARY

The disclosure provides antibodies comprising an antigen-binding variable region that binds specifically to tau. The disclosure, in particular, provides anti-tau antibodies, and antigen-binding fragments thereof, that detect tau in normal (i.e., healthy) human brain tissue, but do not detect tau deposits in human Alzheimer's Disease (AD) brain tissue. The anti-tau antibodies, and antigen-binding fragments thereof, bind to recombinant tau and paired helical filament (“PHF”)-tau by Western assay and do not bind to PHF-tau by ELISA. The antibodies and antigen-binding fragments are capable of specifically binding to a non-phosphorylated tau peptide. The antibodies and antigen-binding fragments are capable of binding to dephosphorylated AD brain tissue.

In certain embodiments, the antibodies and antigen-binding fragments are capable of binding to dephosphorylated AD brain tissue and dephosphorylated PHF-tau. In still other embodiments, the antibodies of the disclosure are non-phospho-selective and do not bind to a peptide phosphorylated at Serine 316. In still other embodiments, the antibodies of the disclosure are non-phospho-selective and do not bind to a peptide phosphorylated at Serine 61 and/or Threonine 63.

In certain embodiments, the disclosure provides chimeric antibodies comprising an antigen-binding variable region from a naturally occurring human antibody that binds specifically to tau, and a recombinant constant region of a human IgG1, wherein the constant region of the chimeric antibody is different from the naturally occurring antibody.

In certain embodiments, the disclosure provides anti-tau antibodies, and antigen-binding fragments thereof, that detect tau in normal human brain tissue, but do not detect tau deposits in human Alzheimer's Disease (AD) and Progressive Supranuclear Palsy (PSP) brain tissue.

In certain embodiments, the chimeric anti-tau antibodies and antigen-binding fragments thereof bind to recombinant tau or PHF-tau by Western assay. In other embodiments, the antibodies and antigen-binding fragments are preferentially capable of specifically binding to a non-phosphorylated-tau peptide.

Preferably, the antibodies are human.

The antibodies and antigen-binding fragments of the disclosure are useful as diagnostic, prophylactic and/or therapeutic agents, both alone and in combination with other diagnostics, prophylactic and/or therapeutic agents.

In one aspect, the disclosure relates to an anti-tau antibody comprising an antigen-binding site comprising a heavy chain CDR1 region of SEQ ID NO:201, a heavy chain CDR2 region of SEQ ID NO:202, and a heavy chain CDR3 region of SEQ ID NO:203, a light chain CDR1 region of SEQ ID NO:204, a light chain CDR2 region of SEQ ID NO:205 and a light chain CDR3 region of SEQ ID NO:206, and to antigen-binding fragments thereof. Another embodiment of the disclosure relates to an anti-tau antibody comprising a heavy chain CDR1 region of SEQ ID NO:207, a heavy chain CDR2 region of SEQ ID NO:208, and a heavy chain CDR3 region of SEQ ID NO:209, a light chain CDR1 region of SEQ ID NO:210, a light chain CDR2 region of SEQ ID NO:211 and a light chain CDR3 region of SEQ ID NO:212, and to antigen-binding fragments thereof. Another embodiment of the disclosure relates to an anti-tau antibody comprising an antigen-binding site comprising a heavy chain CDR1 region of SEQ ID NO:222, a heavy chain CDR2 region of SEQ ID NO:223, and a heavy chain CDR3 region of SEQ ID NO:224, a light chain CDR1 region of SEQ ID NO:225, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:226, and to antigen-binding fragments thereof. Another embodiment of the disclosure relates to an anti-tau antibody comprising an antigen-binding site comprising a heavy chain CDR1 region of SEQ ID NO:238, a heavy chain CDR2 region of SEQ ID NO:239, and a heavy chain CDR3 region of SEQ ID NO:240, a light chain CDR1 region of SEQ ID NO:241, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:242, and to antigen-binding fragments thereof. Another embodiment of the disclosure relates to an anti-tau antibody comprising a heavy chain CDR1 region of SEQ ID NO:243, a heavy chain CDR2 region of SEQ ID NO:244, and a heavy chain CDR3 region of SEQ ID NO:245, a light chain CDR1 region of SEQ ID NO:246, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:212, and to antigen-binding fragments thereof. Another embodiment of the disclosure relates to an anti-tau antibody comprising an antigen-binding site comprising a heavy chain CDR1 region of SEQ ID NO:243, a heavy chain CDR2 region of SEQ ID NO:247, and a heavy chain CDR3 region of SEQ ID NO:248, a light chain CDR1 region of SEQ ID NO:249 a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:212, and to antigen-binding fragments thereof. Another embodiment of the disclosure relates to an anti-tau antibody comprising an antigen-binding site comprising a heavy chain CDR1 region of SEQ ID NO:250, a heavy chain CDR2 region of SEQ ID NO:251, and a heavy chain CDR3 region of SEQ ID NO:252, a light chain CDR1 region of SEQ ID NO:254, a light chain CDR2 region of SEQ ID NO:254 and a light chain CDR3 region of SEQ ID NO:255, and to antigen-binding fragments thereof.

In another aspect, the disclosure relates to an isolated anti-tau antibody comprising an antigen-binding site of a heavy chain variable region (VH) of SEQ ID NOS:115 or 119 or 135 or 147 or 151 or 155 or 159, and an antigen-binding site of a light chain variable region (VL) of SEQ ID NOS:116 or 120 or 136 or 148 or 152 or 156 or 160.

In another aspect, the disclosure relates to an isolated chimeric anti-tau antibody comprising an antigen-binding site of a heavy chain variable region (VH) of SEQ ID NOS:115 or 119 or 135 or 147 or 151 or 155 or 159, and an antigen-binding site of a light chain variable region (VL) of SEQ ID NOS:116 or 120 or 136 or 148 or 152 or 156 or 160. In another aspect of the disclosure, the antibody is non-naturally occurring.

In a further aspect, the disclosure relates to an anti-tau antibody comprising a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:115 and a light chain variable region comprising an amino acid sequence of SEQ ID NO:116 and to antigen-binding fragments thereof. In a further aspect, the disclosure relates to an anti-tau antibody comprising a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:119 and a light chain variable region comprising an amino acid sequence of SEQ ID NO:120 and to antigen-binding fragments thereof. In a further aspect, the disclosure relates to an anti-tau antibody comprising a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:115 and a light chain variable region comprising an amino acid sequence of SEQ ID NO:116 and to antigen-binding fragments thereof. In a further aspect, the disclosure relates to an anti-tau antibody comprising a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:119 and a light chain variable region comprising an amino acid sequence of SEQ ID NO:120 and to antigen-binding fragments thereof. In a further aspect, the disclosure relates to an anti-tau antibody comprising a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:135 and a light chain variable region comprising an amino acid sequence of SEQ ID NO:136 and to antigen-binding fragments thereof. In a further aspect, the disclosure relates to an anti-tau antibody comprising a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:147 and a light chain variable region comprising an amino acid sequence of SEQ ID NO:148 and to antigen-binding fragments thereof. In a further aspect, the disclosure relates to an anti-tau antibody comprising a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:151 and a light chain variable region comprising an amino acid sequence of SEQ ID NO:152 and to antigen-binding fragments thereof. In a further aspect, the disclosure relates to an anti-tau antibody comprising a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:155 and a light chain variable region comprising an amino acid sequence of SEQ ID NO:156 and to antigen-binding fragments thereof. In a further aspect, the disclosure relates to an anti-tau antibody comprising a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:159 and a light chain variable region comprising an amino acid sequence of SEQ ID NO:160 and to antigen-binding fragments thereof.

In one embodiment, the IgG1 heavy chain constant region is comprised of the amino acid sequence of SEQ ID NO:83. In another embodiment, the IgG1 light chain constant region is comprised of the amino acid sequence of SEQ ID NO:84.

The disclosure also provides nucleic acid molecules encoding the antibodies or antigen-binding fragments thereof. Another aspect of the disclosure is a vector comprising the nucleic acid molecules of the disclosure. A further feature of the disclosure is a host cell comprising the vector of the disclosure.

The disclosure also provides a method of producing an anti-tau antibody comprising culturing the host cell of the disclosure and recovering the antibody produced by the host cell.

The disclosure further provides for functional variants of the antibodies and immunoconjugates comprising the antibody and/or antigen-binding fragment thereof.

The disclosure further provides compositions and kits that comprise one or more antibodies of the disclosure and/or antigen-binding fragments thereof. The disclosure additionally provides diagnostic, prophylactic and therapeutic methods that employ the anti-tau antibodies. Prophylactic and therapeutic methods include administering to human subjects the anti-tau antibodies and/or antigen-binding fragments thereof for the prevention or treatment of a tauopathy and/or tau-mediated diseases or conditions, and/or amelioration of one or more symptoms of a tauopathy or tau-mediated disease. Combinations of a plurality of different anti-tau antibodies and/or antigen-binding fragments thereof and/or with other anti-tau antibodies can be used for combination therapy. Compositions comprising the anti-tau antibodies and/or antigen-binding fragments thereof in combination with other prophylactic or therapeutic agents are also provided.

The antibodies of the disclosure are unique in that the variable regions are recovered from anti-tau-specific memory B-cells from healthy individuals and detect tau in normal human brain, but do not detect tau deposits in human Alzheimer's brain. The anti-tau antibodies are also unique in that they bind to denatured PHF-tau in a Western assay, but do not bind to non-denatured PHF-tau in an ELISA. The anti-tau antibodies bind to a non-modified tau peptide 299-369 (SEQ ID NO:331) or a tau peptide 42-103 (SEQ ID NO:325). The chimeric antibodies further bind to a non-modified tau peptide tau 52-71 (SEQ ID NO:382) or tau 299-323 (SEQ ID NO:458) or tau 82-103 (SEQ ID NO:386). The antibodies of the disclosure are unique in that they bind to dephosphorylated AD brain and do not bind to a tau peptide phosphorylated on Serine 316 or Serine 61 or Threonine 63 of tau.

BRIEF DESCRIPTION OF THE DRAWINGS

FIGS. 1A-1T show the reactivity of CBTAU-7.1, 8.1, 16.1, 18.1, 20.1, 22.1, 24.1, 27.1, 28.1, 41.1, 41.2, 42.1, 43.1, 44.1, 45.1, 46.1, 47.1, 47.2, and 49.1 against corresponding cognate and non-cognate peptide.

FIGS. 2A-2J show the reactivity of CBTAU-7.1, 8.1, 16.1, 18.1, 20.1, 22.1, 24.1, 27.1, and 28.1 against recombinant tau (rTau), enriched immunopurified paired helical filaments (ePHF), and immunopurified paired helical filaments (iPHF) by ELISA. Anti-tau mAb, AT8, was used as positive control.

FIG. 3 shows the immunoreactivity of CBTAU-7.1, 18.1, 22.1, 24.1, 27.1, and 28.1 against rTau, ePHF, and iPHF by Western blot analysis.

FIGS. 4A-4G show the epitope mapping of CBTAU-27.1, 28.1, 43.1, 46.1, 47.1, 47.2, and 49.1 using overlapping peptides that correspond to regions 42-103 and 299-369 on human tau441.

FIGS. 5A-5D show the immunohistochemical results for the CBTAU mAbs detailed in this application. FIGS. 5A and 5B show the immunostaining of CBTAU-7.1, 8.1, 16.1, 18.1, 20.1, 22.1, 24.1, 27.1, and 28.1 on non-AD versus AD hippocampal and cortical tissue sections, respectively. FIG. 5C shows the immunostaining of CBTAU-7.1, 8.1, 16.1, 18.1, 20.1, 22.1, and 24.1 on non-PSP and PSP cortical tissue sections. FIG. 5D shows the immunostaining of CBTAU-43.1, 46.1, 47.2, and 49.1 against non-AD and AD cortical tissue sections.

FIG. 6A shows immunoreactivity of CBTAU-28.1 and control mAbs against non-AD (54 y.o. male; no clinical symptoms) and AD (93 y.o. Hispanic female) hippocampal tissue sections.

FIG. 6B shows reactivity of CBTAU-28.1 and control mAbs to AD (93 y.o. Hispanic female) hippocampal tissue sections with and without calf intestinal phosphatase treatment.

FIG. 7 shows reactivity of CBTAU-28.1 and phospho-tau mAb, AT8, against iPHF (immunopurified paired helical filaments) and calf intestinal phosphatase-treated iPHF samples.

FIGS. 8A-8F show reactivity of CBTAU-27.1, 28.1, 43.1, 46.1, 47.1, 47.2, and 49.1 to the tau phosphopeptides detailed on Tables 30-34.

DETAILED DESCRIPTION OF THE INVENTION Definitions

Definitions of terms as used in the disclosure are given below.

The term “included” or “including” as used herein is deemed to be followed by the words “without limitation.”

The term “tau” as used herein, is used interchangeably to specifically refer to the native monomer form of tau. The term “tau” is also used to generally identify other conformers of tau, for example, oligomers or aggregates of tau. The term “tau” is also used to refer collectively to all types and forms of tau. Due to alternative splicing, six tau isoforms are present in the human brain. These isoforms differ by the absence or presence of one or two 29-amino acid inserts encoded by exon 2 and 3 in the amino-terminal part, in combination with either three (R1, R3 and R4) or four (R1-R4) repeat-regions in the carboxy-terminal part. The microtubule-binding domain is encoded by exon 10. The adult tau isoforms include the longest 441-amino acids component (SEQ ID NO:1), or 4R/2N, the 410-amino acids component (SEQ ID NO:2), or 3R/2N, the 412-amino acids component (SEQ ID NO:3), or 4R/1N, the 381-amino acids component (SEQ ID NO:4), or 3R/1N and the 383-amino acids component (SEQ ID NO:5) or 4R/ON. The shortest 352-amino acids isoform (SEQ ID NO:6), or 3R/ON, is found in the fetal brain, and thus is referred to as fetal tau isoform.

The “wild type” tau amino acid sequence is represented by the 441 amino acid isoform (SEQ ID NO:1) also referred to as “tau441,” “4R/2N,” “hTau40,” “TauF,” “Tau-4” or “full-length tau.”

The term “recombinant tau” herein, refers to the longest isoform of human brain tau (SEQ ID NO:1) expressed in E. coli and purified to homogeneity or near homogeneity (S. Barghorn, Meth. Mol. Biol. 2004 299:35-51). Recombinant tau is soluble and is not phosphorylated.

The term “neurofibrillary tangle” (NFT) refers to the pathological structures first described by Alzheimer in the brain of dementia patients. NFT are composed of orderly arranged subunits called paired helical filament aggregates of hyperphosphorylated tau protein that are most commonly known as a primary marker of Alzheimer's Disease.

The term “paired helical filament-tau” or “PHF-tau” as used herein refers to well-known tau aggregates that make up the pathological structures called neurofibrillary tangles (NFT), first described by Alzheimer in the brain of dementia patients. Their presence is also found in numerous other diseases known as tauopathies.

“Enriched PHF-tau” or “ePHF-tau,” is prepared according to the protocol of Greenberg and Davies as detailed in the Examples. PHF-tau is enriched from 27,200×g supernatants containing 0.8 M NaCl by taking advantage of their insolubility in zwitterionic detergents (K. S. Kosik et al. (1986) PNAS USA 83:4044-4048; R. Rubenstein et al. (1986) Brain Res. 372:80-88) and mercaptoethanol. PHFs isolated with zwitterionic detergents appear to maintain antigenic sites that may be lost during the isolation of SDS-insoluble NeuroFibular Tangles and are similar in structure and contain many antigenic properties to PHF in NFTs. “Immunopurified PHF-tau” or “iPHF-tau” is affinity purified with an anti-tau monoclonal antibody. Such protocols have provided PHF-tau preparations that retain the classical paired helical filament structure by electron microscopy and are completely soluble in low concentrations of SDS (G. Jicha, 1997, 48(2):128-32). PHF-tau is also formed from recombinant tau by induction of polymerization in vitro with heparin (Mandelkow, et al., Methods in Molecular Biology 299:35-51(2004). Alternatively, PHF-tau is isolated by various other methods from brains of patients having AD using protocols, such as described in Rostagna and Ghiso (A. Rostagna and J. Ghiso, Curr. Protoc. Cell. Biol. September 2009; CHAPTER: Unit-3.3333). The isolated PHF-tau is characterized for its purity and hyperphosphorylation status with antibodies known to react with PHF-tau. In a typical PHF-tau preparation, the hyperphosphorylated bands migrating at about 60, 64, 68 and 72 kDa in Western blot (Spillantini and Goedert, Trends Neurosci. 21:428-33, 1998) are detected by an AT8 antibody that specifically binds hyperphosphorylated PHF-tau but not dephosphorylated PHF-tau.

The term “antibodies” as used herein is meant in a broad sense and includes immunoglobulin or antibody molecules including polyclonal antibodies, monoclonal antibodies including murine, human, human-adapted, humanized and chimeric monoclonal antibodies, bispecific or multi-specific antibodies and antibody fragments. In general, antibodies are proteins or peptide chains that exhibit binding specificity to a defined antigen. Antibody structures are well known. Immunoglobulins can be assigned to five major classes, namely IgA, IgD, IgE, IgG and IgM, depending on the heavy chain constant domain amino acid sequence. IgA and IgG are further sub-classified as the isotypes IgA1, IgA2, IgG1, IgG2, IgG3 and IgG4. Antibody light chains of any vertebrate species can be assigned to one of two clearly distinct types, namely kappa (κ) and lambda (X), based on the amino acid sequences of their constant domains.

The term “antigen-binding fragments” means a portion of an intact antibody. Examples of antibody fragments include Fab, Fab′, F(ab′)2 and Fv fragments, CDR, antigen-binding site, heavy or light chain variable region, diabodies, triabodies single chain antibody molecules (scFv) and multi-specific antibodies formed from at least two intact antibodies or fragments thereof or (poly) peptides that contain at least a fragment of an immunoglobin that is sufficient to confer antigen binding to the (poly) peptide, etc. An antigen-binding fragment may comprise a peptide or polypeptide comprising an amino acid sequence of at least 2, 5, 10, 15, 20, 25, 30, 35, 40, 50, 60, 70, 80, 90, 100, 125, 150, 175, 200, or 250 contiguous amino acid residues of the amino acid sequence of the antibody. The antigen-binding fragments may be produced synthetically or by enzymatic or chemical cleavage of intact immunoglobulins or they may be genetically engineered by recombinant DNA techniques. The methods of production are well known in the art and are described, for example, in Antibodies: A Laboratory Manual, edited by E. Harlow and D. Lane (1988), Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y., which is incorporated herein by reference. An antibody or antigen-binding fragment thereof may have one or more binding sites. If there is more than one binding site, the binding sites may be identical to one another or they may be different.

An immunoglobulin light or heavy chain variable region consists of a “framework” region interrupted by “antigen-binding sites.” The antigen-binding sites are defined using various terms as follows: (i) Complementarity-Determining Regions (CDRs) are based on sequence variability (Wu and Kabat, J. Exp. Med. 132:211-50, 1970). Generally, the antigen-binding site has three CDRs in each variable region (HCDR1, HCDR2 and HCDR3 in heavy chain variable region (VH) and LCDR1, LCDR2 and LCDR3 in light chain variable region (VL)) (Kabat et al., Sequences of Proteins of Immunological Interest, 5th Ed. Public Health Service, National Institute of Health, Bethesda, Md., 1991). (ii) The term “hypervariable region,” “HVR,” or “HV” refers to the regions of an antibody variable domain that are hypervariable in structure as defined by Chothia and Lesk (Chothia and Lesk, J. Mol. Biol. 96:901-17, 1987). Generally, the antigen-binding site has three hypervariable regions in each VH (H1, H2, H3) and VL (L1, L2, L3). Chothia and Lesk refer to structurally conserved HVs as “canonical structures.” Numbering systems as well as annotation of CDRs and HVs have recently been revised by Abhinandan and Martin (Abhinandan and Martin, Mol. Immunol. 45:3832-9, 2008). (iii) Another definition of the regions that form the antigen-binding site has been proposed by Lefranc (Lefranc, et al., Dev. Camp. Immunol. 27:55-77, 2003) based on the comparison of V domains from immunoglobulins and T-cell receptors. The International ImMunoGeneTics (IMGT) database (http:_//www imgt_org) provides a standardized numbering and definition of these regions. The correspondence between CDRs, HVs and IMGT delineations is described in Lefranc et al. The antigen-binding site can also be delineated based on Specificity-Determining Residue Usage (SDRU) (Almagro, J. Mol. Recognit. 17:132-43, 2004), where Specificity-Determining Residues (SDR), refers to amino acid residues of an immunoglobulin that are directly involved in antigen contact.

Kabat et al. also defined a numbering system for variable domain sequences that is applicable to any antibody. One of ordinary skill in the art can unambiguously assign this system of “Kabat numbering” to any variable domain sequence, without reliance on any experimental data beyond the sequence itself. As used herein, “Kabat numbering” refers to the numbering system set forth by Kabat et al., U.S. Dept. of Health and Human Services, “Sequence of Proteins of Immunological Interest” (1983). Unless otherwise specified, references to the numbering of specific amino acid residue positions in an antibody or antigen-binding fragment, variant, or derivative thereof of the disclosure are according to the Kabat numbering system, which, however, is theoretical and may not equally apply every antibody of the disclosure. For example, depending on the position of the first CDR, the following CDRs might be shifted in either direction.

“Framework” or “framework sequence” are the remaining sequences within the variable region of an antibody other than those defined to be antigen-binding site sequences. Because the exact definition of an antigen-binding site can be determined by various delineations as described above, the exact framework sequence depends on the definition of the antigen-binding site.

The term “monoclonal antibody” (mAb) as used herein means an antibody (or antibody fragment) obtained from a population of substantially homogeneous antibodies. Monoclonal antibodies are highly specific, typically being directed against a single antigenic determinant.

In one aspect, the antibody of the disclosure is a chimeric human antibody. Thus, in accordance with the disclosure, the terms “human chimeric antibody” or “human recombinant antibody” and the like are used to denote a binding molecule, which antigen-binding features originated from a human cell, i.e., which antigen-binding site is derived from nucleic acids produced from a human cell such as a B cell, or the partial cDNA of which has been cloned from mRNA of a human cell, for example, a human memory B cell. A chimeric antibody is still “human” even if amino acid substitutions are made in the antibody, e.g., to improve biophysical or pharmacokinetic characteristics. Compared to artificially generated human-like antibodies such as single chain antibody fragments (scFvs) from a phage displayed antibody library or xenogeneic mice, the chimeric human antibody of the disclosure is characterized by (i) the antigen-binding region being obtained using the human immune response rather than that of animal surrogates, i.e., the antigen-binding region has been generated in response to natural tau in its relevant conformation in the human body, and/or (ii) having protected the individual or is at least significant for the presence of tau.

Antibodies originating from human immunoglobulin libraries or from animals transgenic for one or more human immunoglobulins and that do not express endogenous immunoglobulins, as described infra and, for example, in, U.S. Pat. No. 5,939,598 by Kucherlapati et al., are denoted human-like antibodies in order to distinguish them from human-derived antibodies of the disclosure.

For example, the pairing of heavy and light chains of human-like antibodies such as synthetic and semi-synthetic antibodies typically isolated from phage display do not necessarily reflect the original paring as it occurred in the original human B cell. Accordingly, Fab and scFv fragments obtained from recombinant expression libraries as commonly used in the prior art can be considered as being artificial with all possible associated effects on immunogenicity and stability. In contrast, the disclosure provides antigen-binding regions of affinity-matured anti-tau antibodies from selected human subjects, which, in certain embodiments, are recombinantly expressed as chimeras with a common IgG1 constant region.

The term “functional variant,” as used herein, refers to an antibody that comprises a nucleotide and/or amino acid sequence that is altered by one or more nucleotides and/or amino acids compared to the nucleotide and/or amino acid sequences of a reference antibody and that is capable of competing for specific binding to the binding partner, i.e., tau, with the reference antibody. In other words, the modifications in the amino acid and/or nucleotide sequence of the reference antibody do not significantly affect or alter the binding characteristics of the antibody encoded by the nucleotide sequence or containing the amino acid sequence, i.e., the antibody is still able to specifically recognize and bind its target. The functional variant may have conservative sequence modifications including nucleotide and amino acid substitutions, additions and deletions. Examples of functional variants include de-risking a free Cysteine or amino acid with potential post-translational modification in the hypervariable region, as well as Fc engineering to increase/decrease the binding affinity of IgG antibodies to FcRn, and increase/decrease serum half-life. A functional variant can also be generation of the antibody as a human chimeric IgG2, IgG3 or IgG4 isotype, or as a chimeric isotype of a different species. A functional variant can also be a mutation or mutations of the constant regions for enhancement of bispecific antibody formation. These modifications can be introduced by standard techniques known in the art, such as PCR, site-directed mutagenesis and random PCR-mediated mutagenesis, and may comprise natural as well as non-natural nucleotides and amino acids.

The term “specifically binding” or “specifically recognize,” as used herein, in reference to the interaction of an antibody and its binding partner, e.g., an antigen, means that the interaction is dependent upon the presence of a particular amino acid sequence or structure, e.g., an antigenic determinant or epitope, on the binding partner. In other words, the antibody preferentially binds or recognizes the binding partner, even when the binding partner is present in a mixture of other molecules or organisms. The binding may be mediated by covalent or noncovalent interactions or a combination of both. In yet other words, the term “specifically binding” or “specifically recognizes” means that the antibody is specifically immunoreactive with an antigenic determinant or epitope and is not immunoreactive with other antigenic determinants or epitopes. An antibody that (immuno) specifically binds to an antigen may bind to other peptides or polypeptides with lower affinity as determined by, e.g., radioimmunoassays (MA), enzyme-linked immunosorbent assays (ELISA), BIACORE, or other assays known in the art. Antibodies or fragments thereof that specifically bind to an antigen may be cross-reactive with related antigens, carrying the same epitope. Preferably, antibodies or fragments thereof that specifically bind to an antigen do not cross-react with other antigens.

The term “epitope” as used herein means that part of the antigen that is contacted by the CDR loops of antibody. A “structural epitope” comprises about 15-22 contact residues on the antigen surface and involves many amino acid residues that make contact with a large group of residues on CDRs collectively referred to as the paratope of antibody. Direct contact between epitope and paratope residues is established through electrostatic forces such as hydrogen bonds, salt bridges, van der Waals forces of hydrophobic surfaces and shape complementarity. The interface has also bound water molecules or other co-factors that contribute to the specificity and affinity of antigen-antibody interactions. The binding energy of an antigen-antibody complex is primarily mediated by a small subset of contact residues in the epitope-paratope interface. These “energetic residues” are often located in the center of the epitope-paratope interface and make up the functional epitope. Contact residues in the periphery of the interface make generally minor contributions to the binding energy; their replacements have frequently little effect on the binding with antigen. Thus, the binding or functional activity of an epitope involves a small subset of energetic residues centrally located in the structural epitope and contacted by the specificity-determining CDRs. The assignment of a functional epitope on an antigenic protein can be made using several methods including Alanine scan mutagenesis or by solving the crystal structure of the antigen with the antibody. An epitope can be linear in nature or can be a discontinuous epitope, e.g., a conformational epitope, which is formed by a spatial relationship between non-contiguous amino acids of an antigen rather than a linear series of amino acids. A conformational epitope includes epitopes resulting from folding of an antigen, where amino acids from differing portions of the linear sequence of the antigen come in close proximity in three-dimensional space. For discontinuous epitopes, it may be possible to obtain binding of one or more linear peptides with decreased affinity to a so-called partial epitope, e.g., dispersed at different regions of the protein sequence (M. S. Cragg, (2011) Blood 118 (2):219-20).

As used herein, the term “affinity” refers to a measure of the strength of the binding of an individual epitope or partial epitope with the CDRs of a binding molecule, e.g., an immunoglobulin molecule; see, e.g., Harlow et al., Antibodies: A Laboratory Manual, Cold Spring Harbor Laboratory Press, 2nd ed. (1988) at pages 27-28. As used herein, the term “avidity” refers to the overall stability of the complex between a population of immunoglobulins and an antigen, that is, the functional combining strength of an immunoglobulin mixture with the antigen; see, e.g., Harlow at pages 29-34. Avidity is related to both the affinity of individual immunoglobulin molecules in the population with specific epitopes, and also the valences of the immunoglobulins and the antigen. For example, the interaction between a bivalent monoclonal antibody and an antigen with a highly repeating epitope structure, such as a polymer, would be one of high avidity. The affinity or avidity of an antibody for an antigen can be determined experimentally using any suitable method; see, for example, Berzofsky et al., “Antibody-Antigen Interactions” in Fundamental Immunology, W. E. Paul, Ed., Raven Press New York, N.Y. (1984); J. Kuby, Immunology, W.H. Freeman and Company New York, N Y (1992), and methods described herein. General techniques for measuring the affinity of an antibody for an antigen include ELISA, RIA, and surface plasmon resonance. The measured affinity of a particular antibody-antigen interaction can vary if measured under different conditions, e.g., salt concentration, pH. Thus, measurements of affinity and other antigen-binding parameters, e.g., KD, IC50, are preferably made with standardized solutions of antibody and antigen, and a standardized buffer.

Antibodies or antigen-binding fragments or variants thereof of the disclosure may also be described or specified in terms of their ability to specifically detect the presence of antigen. The term “detect” or “detecting” is used in the broadest sense to include quantitative, semi-quantitative or qualitative measurements of a target molecule. In one aspect, antibodies described herein may only determine the presence or absence of tau polypeptide in a biological sample, e.g., by immunohistochemistry and, thus, the tau polypeptide is detectable or, alternatively, undetectable in the sample as determined by the method.

The term “phospho-specific antibody” or “phospho-dependent antibody” herein used means a specific antibody in which at least part or the entire epitope relies on a phosphorylated amino acid residue. A phospho-specific or phospho-dependent antibody does not detect unphosphorylated antigen. The term “phospho-selective antibody” means a specific antibody that preferentially binds to the phosphorylated residue and has higher affinity to the phosphorylated versus the non-phosphorylated antigen. The term “non-phospho-selective antibody” means a specific antibody that preferentially binds to the non-phosphorylated residue and has higher affinity to the non-phosphorylated versus the phosphorylated antigen. In certain embodiments, the anti-tau antibodies of the disclosure, or antigen-binding fragments thereof, are non-phospho-specific.

The term “polynucleotide” is intended to encompass a singular nucleic acid as well as plural nucleic acids, and refers to an isolated nucleic acid molecule or construct, e.g., messenger RNA (mRNA) or plasmid DNA (pDNA). A polynucleotide may comprise a conventional phosphodiester bond or a non-conventional bond (e.g., an amide bond, such as found in peptide nucleic acids (PNA)). The term “nucleic acid molecule” refers to any one or more nucleic acid segments, e.g., DNA or RNA fragments, present in a polynucleotide. By “isolated” nucleic acid or polynucleotide is intended a nucleic acid molecule, DNA or RNA that has been removed from its native environment. For example, a recombinant polynucleotide encoding an antibody contained in a vector is considered isolated for the purposes of this disclosure.

In certain embodiments, the polynucleotide or nucleic acid is DNA. In the case of DNA, a polynucleotide comprising a nucleic acid that encodes a polypeptide normally may include a promoter and/or other transcription or translation control elements operably associated with one or more coding regions. An operable association is when a coding region for a gene product, e.g., a polypeptide, is associated with one or more regulatory sequences in such a way as to place expression of the gene product under the influence or control of the regulatory sequence(s). Thus, a promoter region would be operably associated with a nucleic acid encoding a polypeptide if the promoter was capable of effecting transcription of that nucleic acid. The promoter may be a cell-specific promoter that directs substantial transcription of the DNA only in predetermined cells. Other transcription control elements, besides a promoter, for example, enhancers, operators, repressors, and transcription termination signals, can be operably associated with the polynucleotide to direct cell-specific transcription. Suitable promoters and other transcription control regions are disclosed herein.

As used herein, the terms “treat” or “treatment” refer to both therapeutic treatment and prophylactic or preventative measures, wherein the object is to prevent or slow down (lessen) an undesired physiological change or disorder, such as the development of Parkinsonism or Alzheimer's Disease. Beneficial or desired clinical results include, but are not limited to, alleviation of symptoms, diminishment of extent of disease, stabilized (i.e., not worsening) state of disease, delay or slowing of disease progression, amelioration or palliation of the disease state, and remission (whether partial or total), whether detectable or undetectable. “Treatment” can also mean prolonging survival as compared to expected survival if not receiving treatment. Those in need of treatment include those already with the condition or disorder as well as those prone to have the condition or disorder or those in which the manifestation of the condition or disorder is to be prevented. A “medicament” as used herein, is an agent used in the treatment of an undesirable physiological change or disorder.

By “subject” or “individual” or “animal” or “patient” or “mammal” is meant any subject, particularly a mammalian subject, e.g., a human patient, for whom diagnosis, prognosis, prevention, or therapy is desired.

DESCRIPTION

Tau is an abundant central and peripheral nervous system protein having multiple well-known isoforms. In the human CNS, six major tau isoforms ranging in size from 352 to 441 exist due to alternative splicing (Hanger, et al., Trends Mol. Med. 15:112-9, 2009). These isoforms differ from each other by the regulated inclusion of 0-2 N-terminal inserts, and 3 or 4 tandemly arranged microtubule-binding repeats, and are referred to as ON3R (SEQ ID NO:6), 1N3R (SEQ ID NO:4), 2N3R (SEQ ID NO:2), ON4R (SEQ ID NO:5), 1N4R (SEQ ID NO:3) and 2N4R (SEQ ID NO:1). The term “recombinant tau” as used herein refers to the tau isoform of SEQ ID NO:1 that is devoid of phosphorylation and other post-translational modifications. The tau protein can be recombinantly expressed in high quantities, for example, in E. coli, baculovirus, mammalian or cell-free systems. “Recombinant tau” may be recombinantly expressed and purified using standard methods. (Barghorn, et al. 2004, Meth. Mol. Biol. 35-51).

Tau binds microtubules and regulates transport of cargo through cells, a process that can be modulated by tau phosphorylation that occurs at many of the 79 potential serine (Ser) and threonine (Thr) phosphorylation sites. Tau is highly phosphorylated during brain development. The degree of phosphorylation declines in adulthood. Some of the phosphorylation sites are located within the microtubule binding domains of tau, and it has been shown that an increase of tau phosphorylation negatively regulates the binding of microtubules. For example, Ser262 and Ser396, which lie within or adjacent to microtubule binding motifs, are hyperphosphorylated in the tau proteins of the abnormal paired helical filaments (PHFs), a major component of the neurofibrillary tangles (NFTs) in the brain of AD patients. PHFs are filamentous aggregates of tau proteins that are abnormally hyperphosphorylated and can be stained with specific anti-tau antibodies and detected by light microscopy. The same holds true for so-called straight tau filaments. PHFs form twisted ribbons consisting of two filaments twisted around one another with a periodicity of about 80 nm. These pathological features are commonly referred to as “tau-pathology,” “tauopathology” or “tau-related pathology.” For a more detailed description of neuropathological features of tauopathies, refer to Lee et al., Annu. Rev. Neurosci. 24 (2001), 1121-1159, and Gotz, Brain. Res. Rev. 35 (2001), 266-286, the disclosure content of which is incorporated herein by reference. Physiological tau protein stabilizes microtubules in neurons. Pathological phosphorylation leads to abnormal tau localization and aggregation, which causes destabilization of microtubules and impaired cellular transport. Aggregated tau is neurotoxic in vitro (Khlistunova et al., J. Biol. Chem. 281 (2006), 1205-1214). The exact neurotoxic species remains unclear, however, as do the mechanism(s) by which they lead to neuronal death. Aggregates of tau can be observed as the main component of neurofibrillary tangles (NFT) in many tauopathies, such as Alzheimer's disease (AD), Frontotemporal dementias, supranuclear palsy, Pick's disease, Argyrophilic grain disease (AGD), corticobasal degeneration, FTDP-17, Parkinson's disease, Dementia pugilistica (reviewed in Gendron and Petrucelli, Mol. Neurodegener. 4:13 (2009)). Besides these observations, evidence emerges that tau-mediated neuronal death can occur even in the absence of tangle formation. Soluble phospho-tau species are present in CSF (Aluise et al., Biochim. Biophys. Acta. 1782 (2008), 549-558). Tau aggregates can transmit a misfolded state from the outside to the inside of a cell and transfer between co-cultured cells (Frost et al., J. Biol. Chem. 284 (2009), 12845-12852).

In addition to the involvement in neurodegenerative tauopathies, observed alterations in tau phosphorylation during and after ischemia/reperfusion and after concussive head injury suggest tau plays a crucial role in neuronal damage and clinical pathophysiology of neurovascular disorders such as ischemic stroke (Zheng et al., J. Cell. Biochem. 109 (2010), 26-29), as well as changes in tau found in chronic traumatic encephalopathy, a tauopathy in concussed athletes and military veterans with Traumatic Brain Injury (TBI).

The anti-tau antibodies disclosed herein specifically bind tau and epitopes thereof and to various conformations of tau and epitopes thereof. For example, disclosed herein are antibodies that specifically bind tau found in normal adult human brain. In one example, a tau antibody disclosed herein binds to tau or an epitope thereof and shows no binding above about three times background for other proteins. An antibody that “specifically binds” or “selectively binds” a tau conformer refers to an antibody that does not bind all conformations of tau, i.e., does not bind at least one other tau conformer such as recombinant tau.

The variable domains of the chimeric anti-tau monoclonal antibodies of this disclosure have origin from a pool of healthy human subjects exhibiting a tau-specific immune response. The tau antibodies of this disclosure may also be called “human-derived antibodies” in order to emphasize that those antibody antigen-binding regions were indeed expressed by the subjects and have not been isolated from, for example, a human immunoglobulin-expressing phage library, which hitherto represented one common method for trying to provide human-like antibodies. For example, the antibodies of this disclosure differ from mAb ATB, MC1, and AT100, in that they are human-derived antibodies.

This disclosure provides monoclonal antibodies, wherein the antibodies a) bind tau in normal human brain tissue and b) do not bind tau in human AD brain tissue. In certain embodiments, the antibodies: a) form an immunological complex with tau in normal (i.e., healthy) human brain tissue, and b) do not form an immunological complex with tau in human AD brain tissue.

Anti-tau antibodies of this disclosure can, for example, be characterized by their binding properties to recombinant tau in an ELISA. Recombinant tau purified from E. coli is highly soluble owing to its hydrophilic character. It lacks phosphorylation of Ser, Thr and Tyr residues characteristic of tau found in tauopathies. In one example, the human anti-tau antibodies disclosed herein specifically bind recombinant tau in an ELISA.

In an embodiment, the anti-tau antibody of the disclosure has been shown to specifically bind to a non-phosphorylated-tau peptide of SEQ ID NO:325 or SEQ ID NO:331 or SEQ ID NO:382 or SEQ ID NO:458 or SEQ ID NO:386. In a further embodiment, the anti-tau antibody of the disclosure has been shown to specifically bind to phosphorylated peptides when the serines at positions 316, 61 or the threonine at position 63 are not phosphorylated.

Thus, in certain embodiments, the anti-tau antibodies disclosed herein specifically bind tau peptide in a peptide ELISA. In one embodiment, an anti-tau antibody binds to a tau peptide, e.g., HVPGGGSVQIVYKPVDLSKVTSKCGSLGNIHHKPGGGQVEVKSEKTDFK DRVQSKIGSLDNITHVPGGGNK (SEQ ID NO:331), corresponding to amino acids 299-369 of tau441. In another embodiment, an anti-tau antibody binds to a tau peptide, e.g., GLKFSPLQTPTEDGSEEPGSETSDAKSTPTAEDVTAPLVDEGAPGKQAAAQPHTEIPEGT TA (SEQ ID NO:325), corresponding to amino acids 42-103 of tau441. In another example, an anti-tau antibody binds to a tau peptide, e.g., TEDGSEEPGSETSDAKSTPT (SEQ ID NO:382), corresponding to amino acids 52-71 of tau441. In another embodiment, an anti-tau antibody binds to a tau peptide, e.g., HVPGGGSVQIVYKPVDLSKVTSKCG (SEQ ID NO:458), corresponding to amino acids 299-323 of tau441. In another example, an anti-tau antibody binds to a tau peptide, e.g., EGAPGKQAAAQPHTEIPEGTTA (SEQ ID NO:386), corresponding to amino acids 82-103 of tau441. The anti-tau antibody of the disclosure is unlike previously disclosed human anti-tau monoclonal antibodies (US 2013/0295021), which have been reported to bind to different tau peptides. Monoclonal antibodies NI-105.4E4, NI-105.4A3 and NI-105.4E4 bind to peptides 329-351+387-397, 337-343, and 35-49 of tau441, respectively.

In certain embodiments, the antibodies of the disclosure are chimeric.

In certain embodiments, the antibody is a chimeric antibody comprising an antigen-binding variable region from a human antibody that binds specifically to tau, and a recombinant constant region of a human IgG1, wherein the chimeric antibody is different from the human antibody.

In certain embodiments, the antibody is a chimeric antibody comprising an antigen-binding variable region from a human antibody that binds specifically to tau, and a recombinant constant region of a human IgG1, wherein the constant region of the chimeric antibody differs from the constant region of the human antibody.

In certain embodiments, the antibody is a chimeric antibody comprising a naturally occurring human antigen-binding variable region that binds specifically to tau, and a recombinant constant region of a human IgG1 antibody.

In certain embodiments, the antibody is a chimeric antibody, wherein the antibody comprises naturally occurring human light and heavy chain variable regions from a human antibody, and recombinant human IgG1 heavy and light chain constant regions.

In certain embodiments, the antibody is a chimeric antibody, wherein the chimeric antibody comprises heavy and light chain variable regions from a naturally occurring human antibody, and recombinant human IgG1 heavy and light chain constant regions.

In certain embodiments, the antibody is a chimeric antibody comprising heavy and light chain variable regions from a human antibody, and recombinant human IgG1 heavy and light chain constant regions.

In certain embodiments, the antibody is a non-naturally occurring variant of a human monoclonal antibody.

In certain embodiments, the antibodies bind to phosphatase-treated tau deposits in human AD brain. Thus, in certain embodiments, the antibodies recognize tau in AD brain following phosphatase treatment. In certain embodiments, the antibodies form an immunological complex with tau deposits in phosphatase-treated human AD tissue.

Anti-tau antibodies of the disclosure can, for example, be characterized by their binding properties to PHF-tau in an ELISA. Anti-PHF-tau antibody clone AT8 binds to PHF-tau and has been used extensively to detect PHF-tau in neurofibrillary tangles in samples from Alzheimer's patients. AT8 is a phospho-specific monoclonal antibody and binds to phosphorylated Ser202 and Thr 205 of PHF-tau and is well-published for use in ELISA, immunohistochemistry, immunoblot, Western blot, and related applications. Clone AT8 recognizes Alzheimer Disease tau, as well as PHF-tau by ELISA and does not bind non-phosphorylated-tau from healthy individuals or recombinant tau. In one embodiment, the anti-tau monoclonal antibody of the disclosure does not bind to PHF-tau by ELISA. In another embodiment, the anti-tau monoclonal antibody of the disclosure binds to dephosphorylated PHF-tau by ELISA.

Anti-tau antibodies of the disclosure can be characterized by their binding properties to PHF-tau and recombinant tau by Western blot. In neurodegenerative disorders, several mechanisms (phosphorylation, ubiquitination, acetylation, oxidation, glycation) are involved in the aggregation of tau proteins into PHF (L. Martin et al., Neurochem. Int. 58(4):458-71, 2011). These pathological tau proteins are visualized by Western blotting as three major bands between 55 and 69 kDa, and a minor band at 74 kDa. Tau 55 results from the phosphorylation of the shortest isoform (SEQ ID NO:6), tau 64 from the phosphorylation of tau variants with one cassette exon (SEQ ID NO:4 and/or SEQ ID NO:5), tau 69 from the phosphorylation of tau variants with two cassette exons (SEQ ID NO:2 and/or SEQ ID NO:3). Phosphorylation of the longest tau isoform (SEQ ID NO:1) induces the formation of the additional hyperphosphorylated tau74 variant. In certain embodiments, the anti-tau antibodies of the disclosure bind to PHF-tau and recombinant tau by Western analysis, and do not bind to PHF-tau by ELISA.

In certain embodiments, the antibody a) binds denatured PHF-tau and b) does not bind non-denatured PHF-tau.

In certain embodiments, the antibody binds phosphatase-treated, non-denatured PHF-tau. In certain embodiments, the antibodies bind with higher affinity to phosphatase-treated PHF-tau than PHF-tau isolated from human donor tissue.

In certain embodiments, the antibody a) binds PHF-tau by Western blot and does not bind PHF-tau by ELISA. In certain embodiments, the antibodies bind PHF-tau isolated from human AD tissue by Western Blot and b) do not bind PHF-tau by ELISA.

In certain embodiments, the antibody binds phosphatase-treated PHF-tau by ELISA. In certain embodiments, the antibodies bind with higher affinity to phosphatase-treated PHF-tau isolated from human AD tissue by ELISA.

Anti-tau antibodies of the disclosure can be utilized in and characterized by immunohistochemistry (IHC) of tissue sections from normal or AD brain. Phospho-tau antibodies, in particular, highlight neurofibrillary pathology with a high degree of sensitivity and specificity, whereas, no detection of tau in normal healthy brain is observed. Clinicopathological studies have demonstrated that phospho-tau deposits or accumulations correspond more closely to clinical signs compared to amyloid-β accumulations, and progress in a stepwise fashion from transentorhinal, to limbic, to isocortical areas, forming the basis for AD staging [R. J. Castellani, et al., Acta Neuropathol. (Berl) 111:503(2006); H. Braak and E. Braak, Acta Neuropathol. (Berl) 82:239 (1991 Tau monoclonal antibodies that are commonly used in immunohistochemistry include AT8 (p202/p205 tau), AT180 (p231 tau), AT270 (p181 tau), AT100 (pT212 and S214), and MC-1, (M. Mercken et al., 1992 Acta Neuropathol. 84:265-272; Zheng-Fischhofer 1998 Eur. J. Biochem. 252:542-552, M. Goedert et. al., 1994 Biochem. J. 301:871-877). In one embodiment, the anti-tau monoclonal antibodies of the disclosure detect tau in normal human brain tissue and do not detect tau deposits in human AD brain tissue. In another example, the anti-tau monoclonal antibodies of the disclosure detect tau deposits in dephosphorylated or phosphatase-treated human AD brain tissue.

Anti-tau antibodies can also be utilized in and characterized by immunohistochemistry of additional tauopathies, including Progressive Supranuclear Palsy, Pick's Disease and others. The pathological filamentous-tau inclusions in PSP are composed of aberrantly phosphorylated-tau proteins, but there is a preferential accumulation of abnormal 4R tau isoforms. A panel of anti-tau monoclonal antibodies, including Alz50, Tau-2, T46, PHF-1, PHF-6, 12E8, PHF-1, RD4 and ATB, has been used to characterize PSP deposits (J. Neuropathol. Exp. Neurol. 1998 (6):588-601). All of the monoclonal antibodies stained intraneuronal and glial inclusions, however, 12E8 and PHF-6 stained with less intensity. These antibodies detect different epitopes of tau, e.g., phospho-specific, isoform-specific, and also detect tau deposits in AD brain. RD3, an anti-tau monoclonal antibody that specifically detects the 3-repeat tau isoform, shows limited IHC detection of PSP, yet intensely stains tau deposits in human AD brain tissue. The limited detection of PSP by this antibody is due to reduced levels of the 3-repeat tau isoform in PSP (R. De Silva et al., Neuropath. and Appl. Neurobio. (2003) 29(3)288-302).

In certain embodiments, the antibody comprises a heavy chain comprising: a) heavy chain CDR1 region of SEQ ID NO:201, a heavy chain CDR2 region of SEQ ID NO:202, and a heavy chain CDR3 region of SEQ ID NO:203, or b) a heavy chain CDR1 region of SEQ ID NO:207, a heavy chain CDR2 region of SEQ ID NO:208, and a heavy chain CDR3 region of SEQ ID NO:209, c) a heavy chain CDR1 region of SEQ ID NO:222, a heavy chain CDR2 region of SEQ ID NO:223, and a heavy chain CDR3 region of SEQ ID NO:224, d) a heavy chain CDR1 region of SEQ ID NO:238, a heavy chain CDR2 region of SEQ ID NO:239, and a heavy chain CDR3 region of SEQ ID NO:240 e) a heavy chain CDR1 region of SEQ ID NO:243, a heavy chain CDR2 region of SEQ ID NO:244, and a heavy chain CDR3 region of SEQ ID NO:245, f) a heavy chain CDR1 region of SEQ ID NO:243, a heavy chain CDR2 region of SEQ ID NO:247, and a heavy chain CDR3 region of SEQ ID NO:248, and g) a heavy chain CDR1 region of SEQ ID NO:250, a heavy chain CDR2 region of SEQ ID NO:251, and a heavy chain CDR3 region of SEQ ID NO:252, a light chain CDR1 region of SEQ ID NO:254, a light chain CDR2 region of SEQ ID NO:254 and a light chain CDR3 region of SEQ ID NO:255.

In certain embodiments, the antibody comprises a light chain comprising: a) a light chain CDR1 region of SEQ ID NO:204, a light chain CDR2 region of SEQ ID NO:205 and a light chain CDR3 region of SEQ ID NO:206, b), a light chain CDR1 region of SEQ ID NO:210, a light chain CDR2 region of SEQ ID NO:211 and a light chain CDR3 region of SEQ ID NO:212, c) a light chain CDR1 region of SEQ ID NO:225, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:226, d) a light chain CDR1 region of SEQ ID NO:241, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:242, e) a light chain CDR1 region of SEQ ID NO:246, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:212, f) a light chain CDR1 region of SEQ ID NO:249 a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:212, and g) a light chain CDR1 region of SEQ ID NO:254, a light chain CDR2 region of SEQ ID NO:254 and a light chain CDR3 region of SEQ ID NO:255.

In certain embodiments, the antibody is selected from the group consisting of: a) an antibody comprising a heavy chain CDR1 region of SEQ ID NO:201, a heavy chain CDR2 region of SEQ ID NO:202, and a heavy chain CDR3 region of SEQ ID NO:203, a light chain CDR1 region of SEQ ID NO:204, a light chain CDR2 region of SEQ ID NO:205 and a light chain CDR3 region of SEQ ID NO:206, b) an antibody comprising a heavy chain CDR1 region of SEQ ID NO:207, a heavy chain CDR2 region of SEQ ID NO:208, and a heavy chain CDR3 region of SEQ ID NO:209, a light chain CDR1 region of SEQ ID NO:210, a light chain CDR2 region of SEQ ID NO:211 and a light chain CDR3 region of SEQ ID NO:212, c) an antibody comprising a heavy chain CDR1 region of SEQ ID NO:222, a heavy chain CDR2 region of SEQ ID NO:223, and a heavy chain CDR3 region of SEQ ID NO:224, a light chain CDR1 region of SEQ ID NO:225, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:226, d) an antibody comprising a heavy chain CDR1 region of SEQ ID NO:238, a heavy chain CDR2 region of SEQ ID NO:239, and a heavy chain CDR3 region of SEQ ID NO:240, a light chain CDR1 region of SEQ ID NO:241, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:242, e) an antibody comprising a heavy chain CDR1 region of SEQ ID NO:243, a heavy chain CDR2 region of SEQ ID NO:244, and a heavy chain CDR3 region of SEQ ID NO:245, a light chain CDR1 region of SEQ ID NO:246, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:212, f) an antibody comprising a heavy chain CDR1 region of SEQ ID NO:243, a heavy chain CDR2 region of SEQ ID NO:247, and a heavy chain CDR3 region of SEQ ID NO:248, a light chain CDR1 region of SEQ ID NO:249 a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:212, and g) an antibody comprising a heavy chain CDR1 region of SEQ ID NO:250, a heavy chain CDR2 region of SEQ ID NO:251, and a heavy chain CDR3 region of SEQ ID NO:252, a light chain CDR1 region of SEQ ID NO:254, a light chain CDR2 region of SEQ ID NO:254 and a light chain CDR3 region of SEQ ID NO:255.

In certain embodiments, the antibody comprises a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:115, a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:119, a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:135, a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:147, a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:151, a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:155, a heavy chain variable region comprising the amino acid sequence of SEQ ID NO:159. In certain embodiments, the antibody comprises a light chain variable region comprising the amino acid sequence of SEQ ID NO:116, a light chain variable region comprising the amino acid sequence of SEQ ID NO:120, comprises a light chain variable region comprising the amino acid sequence of SEQ ID NO:136, a light chain variable region comprising the amino acid sequence of SEQ ID NO:148, comprises a light chain variable region comprising the amino acid sequence of SEQ ID NO:152, a light chain variable region comprising the amino acid sequence of SEQ ID NO:156, comprises a light chain variable region comprising the amino acid sequence of SEQ ID NO:169.

In certain embodiments, the antibodies bind to a peptide selected from the group consisting of SEQ ID NO:325 and SEQ ID NO:331.

In certain embodiments, the antibodies bind to a peptide selected from the group consisting of 382, 458 and 386.

In certain embodiments, the anti-tau antibody of the disclosure has been shown to specifically bind to an epitope comprising D314, L315, and K317 or L315, K317 and P312 or P59, S61, E62, T63, D65, and K67 of tau 441.

In certain embodiments, antigen-binding fragments of the above-described antibodies are provided. The antigen-binding fragments preferably bind to the same epitope. The anti-tau monoclonal antibodies and antigen-binding fragments of the disclosure bind to different epitopes as compared to the epitopes of known human anti-tau antibodies, such as, e.g., NI-105.4E4, and NI-105.4A3. With “binding to a different epitope,” it is meant that the antibody binds to different critical amino acid residues as compared to known antibodies. It has furthermore been shown that the antibodies of the disclosure are non-phospho-selective.

In certain embodiments, the antibodies act synergistically when used in combination with other antibodies binding to tau protein. As used herein, the term “synergistic” means that the combined effect of the antibodies or antigen-binding fragments when used in combination is greater than their additive effects when used individually. A way of calculating synergy is by means of the combination index. The concept of the combination index (CI) has been described by Chou and Talalay (Adv. Enzyme Regul. 22:27-55, 1984).

In certain embodiments, the antibodies and antigen-binding fragments are for use as a medicament, and preferably for use in the diagnostic, therapeutic and/or prophylactic treatment of neurodegenerative diseases. Human anti-tau antibodies of the disclosure or fragments thereof, including Fab, (Fab′)2, scFv fragments, or antibodies comprising antigen-binding sites of the antibodies of the disclosure can be used to treat, reduce or prevent symptoms in patients having a neurodegenerative disease that involves accumulation of tau or pathological tau or tau aggregation within the brain, such as patients suffering from AD as well as any other tauopathy or other tau-related pathologies in which tau may be overexpressed. While not wishing to be bound by any particular theory, the antibodies of the disclosure may exert their beneficial effect by reducing or eliminating pathological tau or tau aggregation and hence the amount of PHF-tau in the brain. The antibodies of the disclosure may be used to treat an animal patient belonging to any classification. Examples of such animals include mammals such as humans, rodents, dogs, cats and farm animals. For example, the antibodies of the disclosure are useful in the preparation of a medicament for treatment of AD wherein the medicament is prepared for administration in dosages defined herein.

Another embodiment of the disclosure is a method of treating or reducing symptoms of a neurodegenerative disease that involves aggregation of tau in a patient comprising administering to the patient a therapeutically effective amount of the isolated antibody of the disclosure for a time sufficient to treat or reduce symptoms of the neurodegenerative disease. Another embodiment of the disclosure is a method of reducing tau in patients in need thereof comprising administering to the patient a therapeutically effective amount of the isolated antibody of the disclosure for a time sufficient to reduce tau.

In any of the embodiments above, the neurodegenerative disease that involves aggregation of tau is a tauopathy. As used herein, a “tauopathy” encompasses any neurodegenerative disease that involves the pathological aggregation of tau within the brain. In addition to familial and sporadic AD, other exemplary tauopathies are frontotemporal dementia with Parkinsonism linked to chromosome 17 (FTDP-17), progressive supranuclear palsy, corticobasal degeneration, Pick's disease, progressive subcortical gliosis, tangle only dementia, diffuse neurofibrillary tangles with calcification, argyrophilic grain dementia, amyotrophic lateral sclerosis, Parkinsonism-dementia complex, Down syndrome, Gerstmann-Straussler Scheinker disease, Hallervorden-Spatz disease, inclusion body myositis, Creutzfeld-Jakob disease, multiple system atrophy, Niemann-Pick disease type C, prion protein cerebral amyloid angiopathy, subacute sclerosing panencephalitis, myotonic dystrophy, nonguanamian motor neuron disease with neurofibrillary tangles, post-encephalitic Parkinsonism, and chronic traumatic encephalopathy, such as dementia pugilistica (boxing disease) (Morris, et al., Neuron. 70:410-26, 2011).

A tauopathy-related behavioral phenotype includes cognitive impairments, early personality change and disinhibition, apathy, abulia, mutism, apraxia, perseveration, stereotyped movements/behaviors, hyperorality, disorganization, inability to plan or organize sequential tasks, selfishness/callousness, antisocial traits, a lack of empathy, halting, agrammatic speech with frequent paraphasic errors but relatively preserved comprehension, impaired comprehension and word-finding deficits, slowly progressive gait instability, retropulsion, freezing, frequent falls, non-levodopa responsive axial rigidity, supranuclear gaze palsy, square wave jerks, slow vertical saccades, pseudobulbar palsy, limb apraxia, dystonia, cortical sensory loss, and tremor.

Patients amenable to treatment include asymptomatic individuals at risk of AD or other tauopathy, as well as patients presently showing symptoms. Patients amenable to treatment include individuals who have a known genetic risk of AD, such as a family history of AD or presence of genetic risk factors in the genome. Exemplary risk factors are mutations in the amyloid precursor protein (APP), especially at position 717 and positions 670 and 671 (Hardy and Swedish mutations, respectively). Other risk factors are mutations in the presenilin genes, PS1 and PS2, and ApoE4, family history of hypercholesterolemia or atherosclerosis. Individuals presently suffering from AD can be recognized from characteristic dementia by the presence of risk factors described above. In addition, a number of diagnostic tests are available to identify individuals who have AD. These include measurement of cerebrospinal fluid tau and A1342 levels. Elevated tau and decreased A1342 levels signify the presence of AD. Individuals suffering from AD can also be diagnosed by AD and Related Disorders Association criteria.

Another embodiment of the disclosure is a method of reducing tau in patients in need thereof comprising administering to the patient a therapeutically effective amount of the isolated anti-tau antibody of the disclosure for a time sufficient to reduce tau. Patients amenable to treatment may suffer from an ailment associated with overexpression of tau. Some mutations, including mutations in intron 10, induce increased levels of the functionally normal four-repeat tau protein isoform, leading to neurodegeneration. Overexpression of the four-repeat human tau protein isoform specifically in neurons in a transgenic mouse led to development of axonal degeneration in brain and spinal cord. In the model, axonal dilations with accumulation of neurofilaments, mitochondria, and vesicles were documented. The axonopathy and the accompanying dysfunctional sensorimotor capacities were transgene-dosage related. These findings proved that merely increasing the concentration of the four-repeat tau protein isoform is sufficient to injure neurons in the central nervous system, without formation of intraneuronal neurofibrillary tangles (Spittaels, et al., Am. J. Pathology 155(6):2153-2165, 1999).

Administration/Pharmaceutical Compositions

Anti-tau antibodies of the disclosure are suitable, both as therapeutic and prophylactic agents for treating or preventing neurodegenerative diseases that involves accumulation of tau, and/or pathological aggregation of tau, such as AD or other tauopathies or tau-associated ailments. In asymptomatic patients, treatment can begin at any age (e.g., at about 10, 15, 20, 25, 30 years). Usually, however, it is not necessary to begin treatment until a patient reaches about 40, 50, 60, or 70 years. Treatment typically entails multiple dosages over a period of time. Treatment can be monitored by assaying antibody, or activated T-cell or B-cell responses to the therapeutic agent over time. If the response falls, a booster dosage is indicated.

In prophylactic applications, pharmaceutical compositions or medicaments are administered to a patient susceptible to, or otherwise at risk of, AD or other ailments involving tau, in an amount sufficient to eliminate or reduce the risk, lessen the severity, or delay the outset of the disease, including biochemical, histologic and/or behavioral symptoms of a disease, its complications and intermediate pathological phenotypes presented during development of the disease. In therapeutic applications, compositions or medicaments are administered to a patient suspected of, or already suffering from, such a disease in an amount sufficient to reduce, arrest, or delay any of the symptoms of the disease (biochemical, histologic and/or behavioral). Administration of a therapeutic may reduce or eliminate mild cognitive impairment in patients that have not yet developed characteristic Alzheimer's pathology. An amount adequate to accomplish therapeutic or prophylactic treatment is defined as a therapeutically or prophylactically effective dose. In both prophylactic and therapeutic regimes, compositions or medicaments are usually administered in several dosages until a sufficient immune response has been achieved.

Anti-tau antibodies or fragments thereof of the disclosure may be administered in combination with other agents that are effective for treatment of related neurodegenerative diseases. In the case of AD, antibodies of the disclosure may be administered in combination with agents that reduce or prevent the deposition of amyloid beta (Aβ). It is possible that PHF-tau and AP pathologies are synergistic. Therefore, combination therapy targeting the clearance of both PHF-tau and AP-related pathologies at the same time may be more effective than targeting each individually.

In the case of Parkinson's Disease and related neurodegenerative diseases, immune modulation to clear aggregated forms of the α-synuclein protein is also an emerging therapy. A combination therapy that targets the clearance of both tau and α-synuclein proteins simultaneously may be more effective than targeting either protein individually. In the methods of the disclosure, the “therapeutically effective amount” of the antibody in the treatment or ameliorating symptoms of a tauopathy can be determined by standard research techniques. For example, the dosage of the antibody can be determined by administering the agent to relevant animal models well known in the art.

In addition, in vitro assays can be optionally employed to help identify optimal dosage ranges. Selection of a particular effective dose can be determined (e.g., via clinical trials) by those skilled in the art based upon the consideration of several factors. Such factors include the disease to be treated or prevented, the symptoms involved, the patient's body mass, the patient's immune status and other factors known by the skilled artisan. The precise dose to be employed in the formulation will also depend on the route of administration, and the severity of disease, and should be decided according to the judgment of the practitioner and each patient's circumstances. Effective doses can be extrapolated from dose-response curves derived from in vitro or animal model test systems. The mode of administration for therapeutic use of the antibodies of the disclosure may be any suitable route that delivers the agent to the host. Pharmaceutical compositions of these antibodies are useful for parenteral administration, e.g., intradermal, intramuscular, intraperitoneal, intravenous, subcutaneous, intranasal or intracranial, or they can be administered into the cerebrospinal fluid of the brain or spine.

The antibodies of the disclosure may be prepared as pharmaceutical compositions containing an effective amount of the antibody as an active ingredient in a pharmaceutically acceptable carrier. The term “carrier” refers to a diluent, adjuvant, excipient, or vehicle with which the antibody is administered. Such pharmaceutical vehicles can be liquids, such as water and oils, including those of petroleum, animal, vegetable or synthetic origin, such as peanut oil, soybean oil, mineral oil, sesame oil and the like. For example, 0.4% saline and 0.3% glycine can be used. These solutions are sterile and generally free of particulate matter. They may be sterilized by conventional, well-known sterilization techniques (e.g., filtration). The compositions may contain pharmaceutically acceptable auxiliary substances as required to approximate physiological conditions such as pH adjusting and buffering agents, stabilizing, thickening, lubricating and coloring agents, etc. The concentration of the antibodies of the disclosure in such pharmaceutical formulation can vary widely, i.e., from less than about 0.5%, usually at or at least about 1% to as much as 15% or 20% by weight and will be selected primarily based on required dose, fluid volumes, viscosities, etc., according to the particular mode of administration selected.

The treatment may be given in a single dose schedule, or as a multiple dose schedule in which a primary course of treatment may be with 1-10 separate doses, followed by other doses given at subsequent time intervals required to maintain and or reinforce the response, for example, at 1-4 months for a second dose, and if needed, a subsequent dose(s) after several months. Examples of suitable treatment schedules include: (i) 0, 1 month and 6 months, (ii) 0, 7 days and 1 month, (iii) 0 and 1 month, (iv) 0 and 6 months, or other schedules sufficient to elicit the desired responses expected to reduce disease symptoms, or reduce severity of disease. Thus, a pharmaceutical composition of the disclosure for intramuscular injection could be prepared to contain 1 ml sterile buffered water, and between about 1 ng to about 100 mg, about 50 ng to about 30 mg or about 5 mg to about 25 mg of an antibody of the disclosure. Similarly, a pharmaceutical composition of the disclosure for intravenous infusion could be made up to contain about 250 ml of sterile Ringer's solution, and about 1 mg to about 30 mg or about 5 mg to about 25 mg of an antibody of the disclosure. Actual methods for preparing parenterally administrable compositions are well known and are described in more detail in, for example, Remington's Pharmaceutical Science, 15th ed., Mack Publishing Company, Easton, Pa.

The antibodies of the disclosure can be lyophilized for storage and reconstituted in a suitable carrier prior to use. This technique has been shown to be effective with antibody and other protein preparations and known lyophilization and reconstitution techniques can be employed.

Diagnostic Methods and Kits

Antibodies of the disclosure may be used in methods of diagnosing AD or other tauopathy in a subject. This method involves detecting, in the subject, the presence of tau using a diagnostic reagent such as an antibody or a fragment thereof of this disclosure. Tau may be detected in a biological sample from a subject (e.g., blood, urine, cerebral spinal fluid) by contacting the biological sample with the diagnostic antibody reagent, and detecting binding of the diagnostic antibody reagent to PHF-tau in the sample from the subject. Assays for carrying out the detection include well-known methods such as ELISA, immunohistochemistry, Western blot, or in vivo imaging. Exemplary diagnostic antibodies are antibodies CBTAU-27.1, CBTAU-28.1, CBTAU-43.1, CBTAU-46.1, CBTAU-47.1, CBTAU-47.2, and CBTAU-49.1 of the disclosure, and are of IgG1, K type.

Diagnostic antibodies or similar reagents can be administered by intravenous injection into the body of the patient, or directly into the brain by any suitable route that delivers the agent to the host as exemplified above. The dosage of antibody should be within the same ranges as for treatment methods. Typically, the antibody is labeled, although in some methods, the primary antibody with affinity for tau is not labeled and a secondary labeling agent is used to bind to the primary antibody. The choice of label depends on the means of detection. For example, a fluorescent label is suitable for optical detection. Use of paramagnetic labels is suitable for tomographic detection without surgical intervention. Radioactive labels can also be detected using PET or SPECT.

Diagnosis is performed by comparing the number, size, and/or intensity of labeled tau, tau accumulation, tau aggregates, and/or neurofibrillary tangles in a sample from the subject or in the subject, to corresponding baseline values. The baseline values can represent the mean levels in a population of non-diseased individuals. Baseline values can also represent previous levels determined in the same subject.

The diagnostic methods described above can also be used to monitor a subject's response to therapy by detecting the presence of tau in a subject before, during or after the treatment. A change in values relative to baseline signals a response to treatment. Values can also change temporarily in biological fluids as pathological tau is being cleared from the brain.

The disclosure is further directed to a kit for performing the above-described diagnostic and monitoring methods. Typically, such kits contain a diagnostic reagent such as the antibodies of the disclosure and, optionally, a detectable label. The diagnostic antibody itself may contain the detectable label (e.g., fluorescent molecule, biotin, etc.), which is directly detectable or detectable via a secondary reaction (e.g., reaction with streptavidin). Alternatively, a second reagent containing the detectable label may be utilized, where the second reagent has binding specificity for the primary antibody. In a diagnostic kit suitable for measuring tau in a biological sample, the antibodies of the kit may be supplied pre-bound to a solid phase, such as to the wells of a microtiter dish.

The contents of all cited references (including literature references, issued patents, published patent applications, and co-pending patent applications) cited throughout this application are hereby expressly incorporated by reference.

EXAMPLES Example 1 Tau Peptide Design and Labeling

Hyperphosphorylation of tau protein resulting in release from microtubules and leading to depolymerization is a pathological hallmark occurring in Alzheimer's disease (AD) and other related tauopathies. As the equilibrium of free tau to microtubule-bound tau shifts in favor of the former, unassociated tau protein is thought to accumulate in a misfolded, aggregated state. During the disease process, tau is thought to adopt a variety of conformations, progressing from soluble dimeric and oligomeric forms to higher-order insoluble aggregates such as paired helical filaments (PHFs) and neurofibrillary tangles (NFTs). However, the exact forms of tau that contribute to pathology and, hence, optimal for therapeutic targeting, remain unknown. Consequently, attempts to target disease-promoting tau are often limited by the choice of target. In an effort to prepare novel anti-tau binding molecules, antibody variable regions to tau were recovered from human memory B-cells using phosphorylated and non-phosphorylated-tau peptides as bait antigens using a single-cell-based approach.

Human memory B-cells to tau are likely rare in the human repertoire; therefore, it was decided to label the tau baits with the brightest fluorophores. All tau peptides were synthesized with an amino-terminal biotin group to aid labeling with two bright fluorophores, streptavidin-APC or streptavidin-PE (aka, tau peptide tetramers). Each tau peptide was labeled with both fluorophores to increase the signal-to-noise during the screening of human memory B-cells (detailed in Example 2) from donor samples. Labeled tau peptide tetramers were prepared by mixing biotinylated peptide at a 35:1 molar ratio of peptide to streptavidin label overnight at 4° C. with gentle mixing. Free peptide was removed by separation over a BioSpin 30 column (Biorad). All tau peptide tetramers were stored at 4° C. for up to 2 months.

Example 2

Recovery of Anti-Tau-Specific Memory B-Cells by FACs Sorting with Labelled Peptide Tetramers

Monoclonal antibodies against tau were recovered from memory B-cells (CD22+CD19+CD27+IgG+) isolated from peripheral blood mononuclear cells (PBMCs) obtained from presumably asymptomatic (non-AD) human blood donors obtained from San Diego Blood Bank and TSRI Normal Blood Donor Services. In addition, AD patient blood samples were obtained through the CRO, Quintiles, from which three antibodies detailed here were recovered. PBMCs were isolated on FICOLL-PAQUE PLUS® (GE Healthcare) and cryopreserved at 50 million cells per ml in 90% FBS and 10% DMSO. An aliquot of plasma was heat inactivated at 56° C. and stored at −20° C. for downstream assessment of plasma reactivity.

For each sorting experiment, PBMCs from three to four donors were thawed and transferred to tubes containing pre-warmed RPMI complete (RPMI, 10% heat inactivated FBS and 1% penicillin/streptomycin), washed and incubated separately at 37° C. for 16 hours. Pooled PBMCs were enriched for mature B-cells by positive selection using CD22+magnetic beads (Miltenyi Biotec). Cells were resuspended in Tris-buffered saline pH 7.4, containing 2 mM EDTA and 0.25% bovine serum albumin Fraction V (IBS Buffer). The cells were stained with the extracellular markers IgG-FITC, CD19-PerCPCy5.5 and CD27-PECy7 (all from BD Biosciences) to label B-cells. Ten million cells were removed and as a negative control, biotin streptavidin-labeled conjugates were used. The remaining cells were incubated with a pool of ten dual-labeled tau peptide tetramers (SA-APC and SA-PE) at 16.8 nM each. Cells were incubated for 60 minutes at 4° C. with gentle mixing, washed twice and re-suspended at 20 million cells per ml in TBS buffer. Prior to sorting, DAPI (Thermo Fisher) was added as a live cell marker and cells were sorted on a Beckman Coulter MoFlo XDP. Negative control samples were used to determine nonspecific binding and signal-to-noise ratio. CD19+, IgG+, CD27hi, and antigen double-positive cells were collected and deposited into individual wells of a 96-well PCR plate and stored at −80° C.

Example 3

Recovery of Heavy and Light Chain Genes from Tau-Specific Single B-Cells

As detailed in Example 2, memory B-cells with reactivity to tau peptide tetramers were identified, isolated and sorted into individual microtiter wells. Heavy and light chain cDNAs were then recovered by a two-step PCR approach from individual B-cells, and variable domain sequences were cloned and expressed in vitro as full-length recombinant IgG1 antibodies and are thus human chimeric antibodies.

First Strand cDNA Synthesis

First-strand complementary DNA (cDNA) was generated from single sorted cells according to manufacturer's protocol (Superscript III, Invitrogen Corp.) with the following modifications: to each well containing a single B-cell, 0.5 μl of 10% NP-40, 1.0 μl of oligo dT, 1.0 μl of dNTP was added and samples were incubated at 65° C. for 5 minutes. After incubation, samples were placed on ice for 1 minute. The following was then added to each well: 2.0 μl of DTT, 4.0 μl of MgCl2, 1.0 μl of SUPERSCRIPT® RT, and 0.5 μl of RNaseOut. Samples were incubated at 50° C. for 50 minutes, followed by incubation at 85° C. for 5 minutes.

Step I Amplification

For the initial PCR (Step I), 2.5 μl of cDNA preparation was used as a template to amplify heavy and kappa or lambda light chains. Primer pools specific to the leader regions of antibody heavy (CB-5′LVH primers, Table 1), kappa light chain (CB-5′LVk primers, Table 2), and lambda light chain (CB-5′ LVlam primers, Table 3) were used. A single reverse primer specific to the CH1 region, CK, and CL regions of the heavy, kappa light and lambda light chains, respectively, were used in the Step I PCR reaction.

TABLE 1 VH STEP I FORWARD PRIMERS SEQ Primer ID DNA SEQUENCE (5′-3′) ID NO: CB-5′LVH1a ATGGACTGGACCTGGAGGTTCCTC  7 CB-5′LVH1b ATGGACTGGACCTGGAGGATCCTC  8 CB-5′LVH1c ATGGACTGGACCTGGAGGGTCTTC  9 CB-5′LVH1d ATGGACTGGACCTGGAGCATCC 10 CB-5′LVH2 GGACATACTTTGTTCCACGCTCCTGC 11 CB-5′LVH3a AGGTGTCCAGTGTCAGGTGCAGC 12 CB-5′LVH3b AGGTGTCCAGTGTGAGGTGCAGC 13 CB-5′LVH3c AGGTGTCCAGTGTCAGGTACAGC 14 CB-5′LVH4 GCAGCTCCCAGATGGGTCCTG 15 CB-5′LVH5 TCAACCGCCATCCTCGCCCTC 16 CB-5′LVH6 GTCTGTCTCCTTCCTCATCTTCCTGC 17 3′CgCH1 GGAAGGTGTGCACGCCGCTGGTC 18

TABLE 2 VK STEP I FORWARD PRIMERS SEQ Primer ID DNA SEQUENCE (5′-3′) ID NO: CB-5′LVk1a ATGAGGGTCCCCGCTCAGCTC 19 CB-5′LVk1b ATGAGGGTCCCTGCTCAGCTC 20 CB-5′LVk1c ATGAGAGTCCTCGCTCAGCTC 21 CB-5′LVk2 TGGGGCTGCTAATGCTCTGG 22 CB-5′LVk3 CCTCCTGCTACTCTGGCTCCCAG 23 CB-5′LVk4 TCTCTGTTGCTCTGGATCTCTGGTGC 24 CB-5′LVk5 CTCCTCAGCTTCCTCCTCCTTTGG 25 CB-5′LVk6 AACTCATTGGGTTTCTGCTGCTCTGG 26 3′Ck-Rev543 GTTTCTCGTAGTCTGCTTTGCTCAGC 27 3′Ck-Rev494 GTGCTGTCCTTGCTGTCCTGCTC 28 3′Ck-Rev GCACTCTCCCCTGTTGAAGCTCTTTG 29

TABLE 3 VL STEP I FORWARD PRIMERS (5′-3′) SEQ Primer ID DNA SEQUENCE (5′-3′) ID NO: CB-5′ L Vlam1 CTCCTCGCTCACTGCACAGG 30 CB-5′ L V1am2 CTCCTCTCTCACTGCACAGG 31 CB-5′ L Vlam3 CTCCTCACTCGGGACACAGG 32 CB-5′ L Vlam4 ATGGCCTGGACCCCTCTCTG 33 CB-5′ L Vlam5 ATGGCATGGATCCCTCTCTTCCTC 34 3′Cl-Rev CACTAGTGTGGCCTTGTTGGCTTG 35

Step II Amplification

For Step II, 2.5 μl of Step I PCR product was used as a template to amplify heavy, and kappa or lambda light chain variable regions. A pool of forward and reverse primers specifically designed to the framework 1 region of antibody heavy chain (pCB-IgG-VH and 3′SalIJH primers, Table 4), kappa light chain (pCB-IgG-VK and 3′Jk primers, Table 5), and lambda light chain (CB-VL and 3′Clam-Step II primers, Table 6) were used to prepare DNA from the variable regions. Furthermore, Step II primers were designed to introduce XbaI (VK and VL forward primers) and XhoI (3′SalIJH primers) restriction sites for downstream cloning. Following the Step II amplification reactions, heavy and light chain variable domain PCR products were run on a 1% agarose gel. Heavy and light chain variable region fragments were purified according to the manufacturer's protocol (Qiagen) and used in the Step III PCR reaction.

TABLE 4 VH STEP II Forward and Reverse Primers SEQ Primer ID DNA SEQUENCE (5′-3′) ID NO: pCB-IgG-VH1a CCTGTCTGGAATTCAGCATGGCCCAGGTGC 36 AGCTGGTGCAGTC pCB-IgG-VH1b CCTGTCTGGAATTCAGCATGGCCCAGGTCC 37 AGCTGGTGCAGTC pCB-IgG-VH1c CCTGTCTGGAATTCAGCATGGCCCAGGTTC 38 AGCTGGTGCAGTC pCB-IgG-VH1d CCTGTCTGGAATTCAGCATGGCCCAGGTCC 39 AGCTTGTGCAGTC pCB-IgG-VH2a CCTGTCTGGAATTCAGCATGGCCCAGGTCA 40 CCTTGAGGGAGTCTGG pCB-IgG-VH2b CCTGTCTGGAATTCAGCATGGCCCAGGTCA 41 CCTTGAAGGAGTCTGG pCB-IgG-VH3a CCTGTCTGGAATTCAGCATGGCCCAGGTGC 42 AGCTGGTGGAGTC pCB-IgG-VH3b CCTGTCTGGAATTCAGCATGGCCGAGGTGC 43 AGCTGTTGGAGTC pCB-IgG-VH3c CCTGTCTGGAATTCAGCATGGCCGAGGTGC 44 AGCTGGTGGAGTC pCB-IgG-VH3d CCTGTCTGGAATTCAGCATGGCCCAGGTAC 45 AGCTGGTGGAGTCTG pCB-IgG-VH4a CCTGTCTGGAATTCAGCATGGCCCAGSTGC 46 AGCTGCAGGAG pCB-IgG-VH4b CCTGTCTGGAATTCAGCATGGCCCAGGTGC 47 AGCTACAGCAGTGG pCB-IgG-VH5 CCTGTCTGGAATTCAGCATGGCCGAGGTGC 48 AGCTGGTGCAGTC pCB-IgG-VH6 CCTGTCTGGAATTCAGCATGGCCCAGGTAC 49 AGCTGCAGCAGTCAG pCB-IgG-VH7 CCTGTCTGGAATTCAGCATGGCCCAGGTGC 50 AGCTGGTGCAATCTG 3′SalIJH TCGGGCCTCGAGACTCACCTGAGGAGACGG 51 1/2/4/5 TGACCAG 3′SalIJH3 TCGGGCCTCGAGACTCACCTGAAGAGACGG 52 TGACCATTG 3′SalIJH6 TCGGGCCTCGAGACTCACCTGAGGAGACGG 53 TGACCGTG

TABLE 5 VK Step II Forward and Reverse Primers SEQ Primer ID DNA SEQUENCE (5′-3′) ID NO: pCB-IgG-VK1a CCGGTCTAGAGTTTTCCATGGCGGACAT 54 CCAGATGACCCAGTCTCC pCB-IgG-VK1b CCGGTCTAGAGTTTTCCATGGCGGACAT 55 CCAGTTGACCCAGTCTCC pCB-IGG-VK1c CCGGTCTAGAGTTTTCCATGGCGGCCAT 56 CCAGTTGACCCAGTCTCC pCB-IGG-VK2a CCGGTCTAGAGTTTTCCATGGCGGATRT 57 TGTGATGACTCAGTCTCCACTC pCB-IgG-VK3a CCGGTCTAGAGTTTTCCATGGCGGAAAT 58 TGTGTTGACGCAGTCTCCAG pCB-IgG-VK3b CCGGTCTAGAGTTTTCCATGGCGGAAAT 59 TGTGTTGACACAGTCTCCAG pCB-IgG-VK3c CCGGTCTAGAGTTTTCCATGGCGGAAAT 60 AGTGATGACGCAGTCTCCAG pCB-IgG-VK4 CCGGTCTAGAGTTTTCCATGGCGGACAT 61 CGTGATGACCCAGTCTCC pCB-IgG-VK5 CCGGTCTAGAGTTTTCCATGGCGGAAAC 62 GACACTCACGCAGTCTCC pCB-IgG-VK6 CCGGTCTAGAGTTTTCCATGGCGGAAAT 63 TGTGCTGACTCAGTCTCCAG 3′Jk1 Rev Ila CGCAAAGTGCACTTACGTTTGATTTCCA 64 CCTTGGTCCCTTGGC 3′Jk2 Rev Iib CGCAAAGTGCACTTACGTTTGATCTCCA 65 GCTTGGTCCCCTGGC 3′Jk4 Rev Ilc CGCAAAGTGCACTTACGTTTGATATCCA 66 CTTTGGTCCCAGGGC 3′Jk3 Rev Ilc CGCAAAGTGCACTTACGTTTGATCTCCA 67 CCTTGGTCCCTCCGC 3′Jk5 Rev Ild CGCAAAGTGCACTTACGTTTAATCTCCA 68 GTCGTGTCCCTTGGC

TABLE 6 VL Step II Forward and Reverse Primers SEQ Primer ID DNA SEQUENCE (5′-3′) ID NO: CB-VL1 CCGGTCTAGAGTTTTCCATGGCGAATTTTATGC 69 TGACTCAGCCCCACTC CB-VL2 CCGGTCTAGAGTTTTCCATGGCGTCCTATGTGC 70 TGACTCAGCC CB-VL3 CCGGTCTAGAGTTTTCCATGGCGCAGTCTGTGC 71 TGACGCAGCC CB-VL4 CCGGTCTAGAGTTTTCCATGGCGCAGTCTGTCG 72 TGACGCAGCC CB-VL5 CCGGTCTAGAGTTTTCCATGGCGCAGTCTGCCC 73 TGACTCAGCC CB-VL6 CCGGTCTAGAGTTTTCCATGGCGTCTTCTGAGC 74 TGACTCAGGACC CB-VL7 CCGGTCTAGAGTTTTCCATGGCGTCCTATGAGC 75 TGACTCAGCCACC 3′Clam- CTCAGAGGAGGGYGGGAACAGAGTGAC 76 Step II

Step III Amplification: Overlap Extension PCR

For Step III, the heavy and light chain variable region DNA fragments produced in Step II were linked into a single cassette via overlap extension PCR using: 1) a kappa linker or lambda linker (see linker preparation method below), which anneals to the 3′ end of the light chain Step II fragment and the 5′ end of the heavy chain Step II fragment, and contains either the kappa or lambda constant region, 2) a forward overlap primer containing an XbaI restriction site, and 3) a reverse primer containing an XhoI restriction site. This reaction results in an approximate 2400 bp or 2200 bp amplicon (i.e., cassette) for the kappa or lambda chains, respectively, consisting of the light chain variable region, linker, and heavy chain variable region. Following amplification, the overlap extension PCR reaction product was PCR-purified according to the manufacturer's instructions (Qiagen PCR Purification Kit).

Linker Preparation

The linker fragment was amplified using pCB-IgG, a dual-CMV promoter vector generated in house and used to express both heavy and light chain genes, as template and the primers listed in Table 7. The linker fragment is 1765 or 1536 base pairs in length for kappa or lambda linker, respectively. The kappa linker contains from a 5′ to 3′ intron sequence followed by the kappa constant region, poly(A) termination sequence, and cytomegalovirus promoter sequence, allowing for one vector expression of the recombinant antibodies. The lambda linker contains the lambda constant region, poly(A) termination sequence, and cytomegalovirus promoter sequence. A common reverse primer (Linker_VH_HAVT20pCB-IgG-R) and kappa-specific forward primer (Linker_CK_intronpCB-IgG-F) were used (Table 7). The amplified fragment was separated on a 1% agarose gel and purified according to the manufacturer's protocol (Qiagen Gel Extraction Kit).

TABLE 7 Linker and Overlap Primers SEQ Primer ID SEQUENCE (5′-3′) ID NO: Linker_VH_HAVT20_ GGCCATGCTGAATTCCAGACAGG 78 pCB-IgG-R Linker_CK_intron_ AAACGTAAGTGCACTTTGCGGCC 79 pCB-IgG-F GCTAGG Linker_CL_intron_ ACTCTGTTCCCRCCCTCCTCTGA 80 pCB-IgG-F_opt GG pCB-overlap F CCGGTCTAGAGTTTTCCATGGCG 81 pCB-overlap R TCGGGCCTCGAGACTCACC 82

Cloning into Mammalian Expression Vector

Following purification of the overlap extension PCR product, the fragment was digested with XhoI and XbaI and subsequently separated on a 1% agarose gel. The band corresponding to the overlap cassette (˜2.4 kb) was purified and ligated into an IgG1 expression vector, pCB-IgG. Antibody variable genes were subcloned into this vector and antibodies were recombinantly expressed as IgG1, regardless of their original (native) isotype. (An example of an IgG1 heavy chain constant region amino acid sequence is shown in SEQ ID NO:83 and light chain kappa constant region amino acid sequence is shown in SEQ ID NO:84.) All transformations were carried out using DH5a Max Efficiency cells (Invitrogen Corp.) and recovered in 250 μl of SOC for 1 hour at 37° C. Approximately 100 μl of recovered cells were plated onto a carbenicillin plate supplemented with 20 mM glucose. Plates were incubated overnight at 37° C. to allow for colony growth. The remaining recovered cell mixture was cultured with 4 ml of Super Broth (SB) media supplemented with 50 μg/ml carbenicillin and incubated overnight at 37° C. with shaking at 250 rpm. The following day, five colonies were picked per plate and grown in 3 ml of SB media supplemented with 50 μg/ml carbenicillin overnight at 37° C. Overnight cultures were used for DNA plasmid preparation (Qiagen).

Example 4 Antibody Sequencing, Germline Identification and Confirmation of Anti-Tau Peptide Reactivity in Transfection Supernatant

To express IgG1s, DNA plasmid minipreps of the aforementioned 4 ml cultures were prepared (Qiagen) and used to transfect 293Expi cells using EXPIFECTAMINE® according to the manufacturer's instructions (Invitrogen, Corp.). Transfections were carried out for a minimum of 72 hours in 10 ml cultures to allow for sufficient IgG1 expression. Cell media was harvested post-transfection and centrifuged to remove the cells and debris. Supernatants were quantified using Protein A sensor tips on an Octet Red system (ForteBio). Each supernatant was subsequently tested by ELISA with the bait peptide in order to confirm the presence of anti-tau reactive antibodies. Plasmid MINIPREP™ DNA (Qiagen) from the four individually picked cultures in Example 3 was prepared and heavy and light chains were sequenced with primers pC9_seq_HC-R (5′CATGTCACCGGGGTGTGG 3′) (SEQ ID NO:85) and pC9_seq_LC-R (5′TCACAGGGGATGTTAGGGACA3′) (SEQ ID NO:86). One clone of the four was selected for subsequent experiments.

Heavy and Light chain variable region protein and nucleic acid sequences of antibody clones CBTAU-7.1 (SEQ ID NOS:87, 88, 89, 90), CBTAU-8.1 (SEQ ID NOS:91, 92, 93, 94), CBTAU-16.1 (SEQ ID NOS:95, 96, 97, 98), CBTAU-18.1 (SEQ ID NOS: 99, 100, 101, 102), CBTAU-20.1 (SEQ ID NOS:103, 104, 105, 106), CBTAU-22.1 (SEQ ID NOS:107, 108, 109, 110), CBTAU-24.1 (SEQ ID NO:111, 112, 113, 114), CBTAU-27.1 (SEQ ID NOS:115, 116, 117, 118), CBTAU-28.1 (SEQ ID NOS:119, 120, 121, 122), CBTAU-41.1 (SEQ ID NOS:123, 124, 125, 126), CBTAU-41.2 (SEQ ID NOS:127, 128, 129, 130), CBTAU-42.1 (SEQ ID NOS:131, 132, 133, 134), CBTAU-43.1 (SEQ ID NOS:135, 136, 137, 138), CBTAU-44.1 (SEQ ID NOS:139, 140, 141, 142), CBTAU-45.1 (SEQ ID NOS:143, 144, 145, 146), CBTAU-46.1 (SEQ ID NOS:147, 148, 149, 150), CBTAU-47.1 (SEQ ID NOS:151, 152, 153, 154), CBTAU-47.2 (SEQ ID NOS:155, 156, 157, 158), and CBTAU-49.1 (SEQ ID NOS:159, 160, 161, 162) define novel CDRs for the selected anti-tau antibodies (Table 8).

An anti-tau antibody CBTAU-7.1 was generated comprising the VH of SEQ ID NO:87 and the VL of SEQ ID NO:88 and a human IgG1 constant region. An anti-tau antibody CBTAU-8.1 was generated comprising the VH of SEQ ID NO:91 and the VL of SEQ ID NO:92 and a human IgG1 constant region. An anti-tau antibody CBTAU-16.1 was generated comprising the VH of SEQ ID NO:95 and the VL of SEQ ID NO:96 and a human IgG1 constant region. An anti-tau antibody CBTAU-18.1 was generated comprising the VH of SEQ ID NO:99 and the VL of SEQ ID NO:100 and a human IgG1 constant region. An anti-tau antibody CBTAU-20.1 was generated comprising the VH of SEQ ID NO:103 and the VL of SEQ ID NO:104 and a human IgG1 constant region. An anti-tau antibody CBTAU-22.1 was generated comprising the VH of SEQ ID NO:107 and the VL of SEQ ID NO:108 and a human IgG1 constant region. An anti-tau antibody CBTAU-24.1 was generated comprising the VH of SEQ ID NO:111 and the VL of SEQ ID NO:112 and a human IgG1 constant region. An anti-tau antibody CBTAU-27.1 was generated comprising the VH of SEQ ID NO:115 and the VL of SEQ ID NO:116 and a human IgG1 constant region. An anti-tau antibody CBTAU-28.1 was generated comprising the VH of SEQ ID NO:119 and the VL of SEQ ID NO:120 and a human IgG1 constant region. An anti-tau antibody CBTAU-41.1 was generated comprising the VH of SEQ ID NO:123 and the VL of SEQ ID NO:124 and a human IgG1 constant region. An anti-tau antibody CBTAU-41.2 was generated comprising the VH of SEQ ID NO:127 and the VL of SEQ ID NO:128 and a human IgG1 constant region. An anti-tau antibody CBTAU-42.1 was generated comprising the VH of SEQ ID NO:131 and the VL of SEQ ID NO:132 and a human IgG1 constant region. An anti-tau antibody CBTAU-43.1 was generated comprising the VH of SEQ ID NO:135 and the VL of SEQ ID NO:136 and a human IgG1 constant region. An anti-tau antibody CBTAU-44.1 was generated comprising the VH of SEQ ID NO:139 and the VL of SEQ ID NO:140 and a human IgG1 constant region. An anti-tau antibody CBTAU-45.1 was generated comprising the VH of SEQ ID NO:143 and the VL of SEQ ID NO:144 and a human IgG1 constant region. An anti-tau antibody CBTAU-46.1 was generated comprising the VH of SEQ ID NO:147 and the VL of SEQ ID NO:148 and a human IgG1 constant region. An anti-tau antibody CBTAU-47.1 was generated comprising the VH of SEQ ID NO:151 and the VL of SEQ ID NO:152 and a human IgG1 constant region. An anti-tau antibody CBTAU-47.2 was generated comprising the VH of SEQ ID NO:155 and the VL of SEQ ID NO:156 and a human IgG1 constant region. An anti-tau antibody CBTAU-49.1 was generated comprising the VH of SEQ ID NO:159 and the VL of SEQ ID NO:160 and a human IgG1 constant region.

TABLE 8 Amino acid sequences of heavy and light chain variable region CDRs Tau aa Clone region CDR1 (SEQ ID NO: ) CDR2 (SEQ ID NO: ) CDR3 (SEQ ID NO: ) CBTAU 194-212 SYWMH RINSDGSDTNYADSVKG GRSYGFFDY 7.1 (163) (164) (165) RASQIISSNYLA GASSRAT QQYGTSPRT (166) (167) (168) CBTAU 194-212 TYGMH VIWFDGNNKYYADSVKG DWWEAGCRPCYFFDY 8.1 (169) (170) (171) KSSQSVLYSSNNKNYLA WASTRES QQYYSPPLT (172) (173) (174) CBTAU 204-221 SYWMS NINQDGSAAYYVDSVRG DAHYYDRNRNNYYYYFDF 16.1 (175) (176) (177) RASQSVGANLA SASTRAT QQYNNWPRT (178) (179) (180) CBTAU 200-217 SGNYYWS RMSSSGSTNYNPSLKS ESGSSWQNHYYYYGMDV 18.1 (181) (182) (183) KSSQSVLYSSNNKNYLA WASTRES QQYYSTPLT (172) (173) (184) CBTAU 58-78 NYAMS GISSDGNTFYADSVKG ESGRWGGGTLYGAHY 20.1 (185) (186) (187) KSSQSLLYNSNNKNYLT WASTRES QQYYSSPLT (188) (173) (189) CBTAU 406-429 DYNVH RISPNSGGTKYAQKFQG GHCDGTTCSRAY 22.1 (190) (191) (192) RSSQSLLHRSGHKYLH LGSNRAS MQTLQTPWT (193) (194) (195) CBTAU 221-245 GYYLH WVNPRSGGTSYPPKFQG GRIPDVTAFDI 24.1 (196) (197) (198) KSSESLLYDSNNKNYLA WASTRES QQYFSTPWT (199) (173) (200) CBTAU 299-328 SYWTA IIYSGDSDTRYHPSVQG LDARVDAGWQLDS 27.1 (201) (202) (203) KSSQSVFSRDNNKNYLA WASSRES QHYFNTPHN (204) (205) (206) CBTAU 52-71 NYWIG IIHPGDSDTRYSPPFQG VGRPSKGGWFDP 28.1 (207) (208) (209) ESSQTLLYSSNEKNYLA WASTPES QQYYNSPYT (210) (211) (212) CBTAU 406-429 DSYMS YISRSSSHTNYADSVKG VQTTMIEGKTKLNYFDY 41.1 (213) (214) (215) ESSHSLLYRSNNRNYLA WASTRES QQFYTTPYT (216) (173) (217) CBTAU 406-429 DSYMS YISRSSSHTNYADSVKG VQTTMIEGKTKLNYFDY 41.2 (213) (214) (215) ESSHSLLYRSNNKNYLA WASTRES QQFYTTPYT (218) (173) (217) CBTAU 406-429 KAWMS RIKSKVDGETTDYAAPVRG LIHCDLSACLPHF 42.1 (219) (220) (221) ESSHSLLYRSNNKNYLA WASTRES QQFYTTPYT (218) (173) (217) CBTAU 299-328 NYWIA IIYPGDSDTTYSPSFQG LPRTDGDNSIGYFEY 43.1 (222) (223) (224) KSSQSVLYSSNSENYLA WASTRES QQYYSTPFT (225) (173) (226) CBTAU 406-429 SYSMN YISSSTTTIYYADSVKG VPAPRLGGSYTY 44.1 (227) (228) (229) RASQSVSSSYLA GASSRAT QQYGTSPLT (230) (167) (231) CBTAU 406-429 DAWMS RIKSKNVGETTDYAEHVRG GLGGGTYG 45.1 (232) (233) (234) RSSAGLRNNDGDILLS RVSRRDS MRGPY (235) (236) (237) CBTAU  82-103 IYEMN YITNRGSTIYYADSVKG PRIGARVFDV 46.1 (238) (239) (240) KSSQTLLYKSNNENYLA WASTRES QQYFTTALT (241) (173) (242) CBTAU 52-71 DHWIG IIFPEDSDTRYSGSFEG VSVVRKGGWFDP 47.1 (243) (244) (245) KSSQSLLYTSNNKNYLA WASTRES QQYYNSPYT (246) (173) (212) CBTAU 52-71 DHWIG IIFPGDSDIRYSPSFEG VAVVRKGGWFDS 47.2 (243) (247) (248) KSTQSLLWSANNKNYLA WASTRES QQYYNSPYT (249) (173) (212) CBTAU 52-71 SYWIG IIYPDDSDTRYNASLEG RDRNCSGTTCYPRWFDS 49.1 (250) (251) (252) KSSQSLFYSGNSKDFLA WASTRDS HQYHSTPLS (253) (254) (255)

CBTAU-7.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:163, a heavy chain CDR2 region of SEQ ID NO:164, and a heavy chain CDR3 region of SEQ ID NO:165, a light chain CDR1 region of SEQ ID NO:166, a light chain CDR2 region of SEQ ID NO:167 and a light chain CDR3 region of SEQ ID NO:168. CBTAU-8.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:169, a heavy chain CDR2 region of SEQ ID NO:170, and a heavy chain CDR3 region of SEQ ID NO:171, a light chain CDR1 region of SEQ ID NO:172, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:174. CBTAU-16.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:175, a heavy chain CDR2 region of SEQ ID NO:176, and a heavy chain CDR3 region of SEQ ID NO:177, a light chain CDR1 region of SEQ ID NO:178, a light chain CDR2 region of SEQ ID NO:179 and a light chain CDR3 region of SEQ ID NO:180. CBTAU-18.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:181, a heavy chain CDR2 region of SEQ ID NO:182, and a heavy chain CDR3 region of SEQ ID NO:183, a light chain CDR1 region of SEQ ID NO:172, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:184. CBTAU-20.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:185, a heavy chain CDR2 region of SEQ ID NO:186, and a heavy chain CDR3 region of SEQ ID NO:187, a light chain CDR1 region of SEQ ID NO:188, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:189. CBTAU-22.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:190, a heavy chain CDR2 region of SEQ ID NO:191, and a heavy chain CDR3 region of SEQ ID NO:192, a light chain CDR1 region of SEQ ID NO:193, a light chain CDR2 region of SEQ ID NO:194 and a light chain CDR3 region of SEQ ID NO:195. CBTAU-24.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:196, a heavy chain CDR2 region of SEQ ID NO:197, and a heavy chain CDR3 region of SEQ ID NO:198, a light chain CDR1 region of SEQ ID NO:199, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:200. CBTAU-27.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:201, a heavy chain CDR2 region of SEQ ID NO:202, and a heavy chain CDR3 region of SEQ ID NO:203, a light chain CDR1 region of SEQ ID NO:204, a light chain CDR2 region of SEQ ID NO:205 and a light chain CDR3 region of SEQ ID NO:206. CBTAU-28.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:207, a heavy chain CDR2 region of SEQ ID NO:208, and a heavy chain CDR3 region of SEQ ID NO:209, a light chain CDR1 region of SEQ ID NO:210, a light chain CDR2 region of SEQ ID NO:211 and a light chain CDR3 region of SEQ ID NO:212. CBTAU-41.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:213, a heavy chain CDR2 region of SEQ ID NO:214, and a heavy chain CDR3 region of SEQ ID NO:215, a light chain CDR1 region of SEQ ID NO:216, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:217. CBTAU-41.2 antibody comprises a heavy chain CDR1 region of SEQ ID NO:213, a heavy chain CDR2 region of SEQ ID NO:214, and a heavy chain CDR3 region of SEQ ID NO:215, a light chain CDR1 region of SEQ ID NO:218, a light chain CDR2 region of SEQ ID NO:174 and a light chain CDR3 region of SEQ ID NO:217. CBTAU-42.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:219, a heavy chain CDR2 region of SEQ ID NO:220, and a heavy chain CDR3 region of SEQ ID NO:221, a light chain CDR1 region of SEQ ID NO:218, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:217. CBTAU-43.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:222, a heavy chain CDR2 region of SEQ ID NO:223, and a heavy chain CDR3 region of SEQ ID NO:224, a light chain CDR1 region of SEQ ID NO:225, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:226. CBTAU-44.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:227, a heavy chain CDR2 region of SEQ ID NO:228, and a heavy chain CDR3 region of SEQ ID NO:229, a light chain CDR1 region of SEQ ID NO:230, a light chain CDR2 region of SEQ ID NO:167 and a light chain CDR3 region of SEQ ID NO:231. CBTAU-45.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:232, a heavy chain CDR2 region of SEQ ID NO:233, and a heavy chain CDR3 region of SEQ ID NO:234, a light chain CDR1 region of SEQ ID NO:235, a light chain CDR2 region of SEQ ID NO:236 and a light chain CDR3 region of SEQ ID NO:237. CBTAU-46.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:238, a heavy chain CDR2 region of SEQ ID NO:239, and a heavy chain CDR3 region of SEQ ID NO:240, a light chain CDR1 region of SEQ ID NO:241, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:242. CBTAU-47.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:243, a heavy chain CDR2 region of SEQ ID NO:244, and a heavy chain CDR3 region of SEQ ID NO:245, a light chain CDR1 region of SEQ ID NO:246, a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:212. CBTAU-47.2 antibody comprises a heavy chain CDR1 region of SEQ ID NO:243, a heavy chain CDR2 region of SEQ ID NO:247, and a heavy chain CDR3 region of SEQ ID NO:248, a light chain CDR1 region of SEQ ID NO:249 a light chain CDR2 region of SEQ ID NO:173 and a light chain CDR3 region of SEQ ID NO:212. CBTAU-49.1 antibody comprises a heavy chain CDR1 region of SEQ ID NO:250, a heavy chain CDR2 region of SEQ ID NO:251, and a heavy chain CDR3 region of SEQ ID NO:252, a light chain CDR1 region of SEQ ID NO:254, a light chain CDR2 region of SEQ ID NO:254 and a light chain CDR3 region of SEQ ID NO:255.

Nucleic acid sequences of heavy and light chain variable regions of the anti-tau monoclonal antibodies were compared to known germline sequences using IgBLAST, an immunoglobulin variable domain sequence analysis tool, available at the NCBI (Nucleic Acids Res. 2013 July; 41 (Web Server issue):W34-40). Sequence alignment of heavy and light chain framework H1 and L1 regions, aligned with their respective proposed germline sequence and PCR primer, are shown in Table 9. Confirmed sequences were scaled up for expression and purification (detailed in Example 5). Selected clones were expanded into a 50 ml culture and plasmid midiprep DNA was prepared (Machery Nagel Midi Prep kit). Plasmid DNA was then used to transfect a 30 ml culture of 293Expi cells as detailed in Example 5.

TABLE 9 Framework nucleic acids of H1 and L1 aligned  with germline and primer (Amino acids above) Differences marked in  lower case lettering. Native refers to the antibody SEQ ID Amino Terminal Protein and N- mAb NO terminal Nucleic Acid Sequences CBTAU-7.1 VH  87 (Q V Q L V E S) pCB-IgG-  37 CAGGTCCAGCTGGTGCAGTC VH1b CBTAU-7.1  89 CAGGTCCAGCTGGTGGAGTCCGGGGGAGGCTT VH AGTTCAGCCTGGGGGGTCCCTGAGACTCTCCT IGHV3- 256 gAGGTgCAGCTGGTGGAGTCCGGGGGAGGCTT 74*01. AGTTCAGCCTGGGGGGTCCCTGAGACTCTCCT Native 7.1 257 (e V Q L V E) VH VL  88 (D I V M T Q S P) pCB-IgG-  61 GACATCGTGATGACCCAGTCTCC Vk4 CBTAU-7.1  90 GACATCGTGATGACCCAGTCTCCAGACACCCT VL GTCTTTGTCTCCAGGGGAGAGAGCCACCCTCT IGKV3- 258 GAaATtGTGtTGACgCAGTCTCCAGcCACCCT NL5*01 GTCTTTGTCTCCAGGGGAaAGAGCCACCCTCT Native 7.1 259 (e I V l T Q S P) VL CBTAU-8.1 VH  91 (Q V A L V E S) pCB-IgG-  42 CAGGTGCAGCTGGTGGAGTC VH3a CBTAU-8.1  93 CAGGTGCAGCTGGTGGAGTCGAGGGGAGGCGT VH GGTCCAGCCTGGGACGTCCCTGAGACTCTCCT IGHV3- 260 CAGGTGCAGCTGGTGGAGTCtgGGGGAGGCGT 33*01 GGTCCAGCCTGGGACGTCCCTGAGACTCTCCT Native 8.1 261 (Q V A L V E S) VH VL  92 (E T T L T Q S P) pCB-IgG-  62 GAAACGACACTCACGCAGTCTCC Vk5 CBTAU-8.1  94 GAAACGACACTCACGCAGTCTCCAGACTCCCT VL GGCTGTGTCTCTGGGCGAGAGGGCCACCATCA IGKV4- 262 GAcAtcgtgaTgACcCAGTCTCCAGACTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGCCACCATCA Native 8.1 263 (d i v m T Q S P) VL CBTAU-16.1 VH  95 (E V Q L V Q) pCB-IgG-  48 GAGGTGCAGCTGGTGCAGTC VH5 CBTAU-  97 GAGGTGCAGCTGGTGCAGTCTGGGGGAGGCTT 16.1 VH GGTCCAGCCTGGGGGGTCCCTGAGACTCTCCT IGHV3- 264 GAGGTGCAGCTGGTGgAGTCTGGGGGAGGCTT 64*01 GGTCCAGCCTGGGGGGTCCCTGAGACTCTCCT Native 265 (E V Q L V e S) 16.1 VH VL  96 (E I V M T Q S P) pCB-IgG-  60 GAAATAGTGATGACGCAGTCTCCGG VK3c CBTAU-  98 GAAATAGTGATGACGCAGTCTCCGGCCACCCT 16.1 VL GTCTGTGTCTCCAGGGGAAAGAGCCACCCTCT IGKV3- 266 GAAATAGTGATGACGCAGTCTCCaGCCACCCT 15*01 GTCTGTGTCTCCAGGGGAAAGAGCCACCCTCT Native 267 (E I V M T Q S P) 16.1 VL CBTAU-18.1 VH  99 (Q V Q L L E S) No exact primer match CBTAU- 101 CAGGTGCAGCTGTTGGAGTCGGGCCCAGGACT 18.1 VH GGTGAACCCTTCACAGACCCTGTCCCTCACCT IGHV4- 268 CAGGTGCAGCTGcaGGAGTCGGGCCCAGGACT 31*05 GGTGAAGCCTTCACAGACCCTGTCCCTCACCT Native 269 (Q V Q L q E S) 18.1 VH VL 100 (E I V L T Q S P) pCB-IgG-  59 GAAATTGTGTTGACACAGTCTCCAG VK3b CBTAU- 102 GAAATTGTGTTGACACAGTCTCCAGACTCCCT 18.1 VL GGCTGTGTCTCTGGGCGAGAGGGCCAACATTA IGKV4- 262 GAcATcGTGaTGACcCAGTCTCCAGACTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGCCAcCATcA Native 270 (d I V m T Q S P) 18.1 VL CBTAU-20.1 VH 103 (Q V Q L V E S) pCB-IgG-  45 CAGGTACAGCTGGTGGAGTCTG VH3d CBTAU- 105 CAGGTACAGCTGGTGGAGTCTGGGGGAGGCTT 20.1 VH GGTACAGCCTGGGGGGTCCCTGAGACTCTCCT IGHV3- 271 gAGGTgCAGCTGGTGGAGTCTGGGGGAGGCTT 23*04 GGTACAGCCTGGGGGGTCCCTGAGACTCTCCT Native 272 (e V Q L V E S) 20.1 VH VL 104 (D I Q M T Q S P) pCB-IgG-  54 GACATCCAGATGACCCAGTCTCC VK1a CBTAU- 106 GACATCCAGATGACCCAGTCTCCAGACTCCCT 20.1 VL GGCTGTGTCTCTGGGCGAGAGGGCCACCATCA IGKV4- 262 GACATCgtGATGACCCAGTCTCCAGACTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGCCACCATCA Native 273 (D I v M T Q S P) 26.1 VL CBTAU-22.1 VH 107 (Q V Q L V Q S) pCB-IgG-  36 CAGGTGCAGCTGGTGCAGTC VH1a CBTAU- 109 CAGGTGCAGCTGGTGCAGTCTGGGGCTGAGGT 22.1 VH GAAGAAGCCTGGGGCCCCAGTGAAGGTCTC IGHV1- 274 CAGGTGCAGCTGGTGCAGTCTGGGGCTGAGGT 2*02 GAAGAAGCCTGGGGCCtCAGTGAAGGTCTC Native 275 (Q V Q L V Q S) 22.1 VH VL 108 (D V V M T Q S P L) No Exact Primer match CBTAU- 110 GATGTTGTGATGACGCAGTCTCCACTCTCCCT 22.1 VL GCCCGTCACCCCTGGAGAGCCGGCCTCCATC IGKV2- 276 GATaTTGTGATGACtCAGTCTCCACTCTCCCT 28*01 GCCCGTCACCCCTGGAGAGCCGGCCTCCATC Native 277 (D i V M T Q S P L) 22.1 VL CBTAU-24.1 VH 111 (Q V Q L V S G) pCB-IgG-  39 CAGGTCCAGCTTGTGCAGTC VH1d CBTAU- 113 CAGGTCCAGCTTGTGCAGTCTGGGGCTGAGGT 24.1 VH GAAGAAGCCTGGGGCCTCAGTGAAGGTCTCC IGHV1- 278 CAGGTCCAGCTTGTGCAGTCTGGGGCTGAGGT 3*01 GAAGAAGCCTGGGGCCTCAGTGAAGGTtTCC Native 279 (Q V Q L V S G) 24.1 VH VL 112 (D I Q M T Q S P) pCB-IgG-  54 GACATCCAGATGACCCAGTCTCC VK1a CBTAU- 114 GACATCCAGATGACCCAGTCTCCAGACTCCCT 24.1 VL GGCTGTGTCTCTGGGCGAGAGGGCCACCATC IGKV4- 262 GACATCgtGATGACCCAGTCTCCAGACTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGCCACCATC Native 280 (D I v M T Q S P) 24.1 VL CBTAU27.1 VH 115 (Q V Q L V E S) pCB-IgG-  42 CAGGTGCAGCTGGTGGAGTC VH3a CBTAU27.1 117 CAGGTTCAGCTGGTGGAGTCTGGACCGGAGAT VH GAGAAAGCCCGGGGAGTCTCTGAAAATTTCC IGHV5- 281 gAGGTgCAGCTGGTGcAGTCTGGAgCaGAGgT 51*01 GAaAAAGCCCGGGGAGTCTCTGAAgATcTCC Native 282 (e V Q L V q S) 27.1 VH VL 116 (D I Q L T Q S P) pCB-IgG-  55 GACATCCAGTTGACCCAGTCTCC VK 1b CBTAU27.1 118 GACATCCAGTTGACCCAGTCTCCAGATTCCCT VL GGCTGTGTCTCTGGGCGAGCGGGCCACCATC IGKV4- 262 GACATCgtGATGACCCAGTCTCCAGACTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGCCACCATC Native 283 (D I v m T Q S)P 27.1 VL CBTAU28.1 VH 119 (Q V Q L Q Q S) pCB-IgG-  49 CAGGTaCAGCTgCAGCAGTCAG VH6 CBTAU28.1 121 CAGGTGCAGCTACAGCAGTCAGGAGCAGAAGT VH GAAAAAGCCCGGGGAGTCTCTGAAGATCTCC IGHV5- 281 gAGGTGCAGCTggtGCAGTCtGGAGCAGAAGT 51*01 GAAAAAGCCCGGGGAGTCTCTGAAGATCTCC Native 284 (e V Q L v Q S) 28.1 VH VL 120 (D I Q M T Q S P) pCB-IgG-  54 GACATCCAGATGACCCAGTCTCC VK1a CBTAU28.1 122 GACATCCAGATGACCCAGTCTCCAGACTCCCT VL GGCTGTGTCTCTGGGCGAGAGGGCCACCATC IGKV4- 262 GACATCgtGATGACCCAGTCTCCAGACTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGCCACCATC Native 285 (D I v M T Q S P) 28.1 VL CBTAU41.1 VH 123 (E V Q L L E S) pCB-IgG-  43 GAGGTGCAGCTGTTGGAGTC VH3b CBTAU41.1 125 GAGGTGCAGCTGTTGGAGTCTGGGGGAGGCTT VH GGTCAAGCCTGGAGGGTCCCTGAGACTCTCC IGHV3- 286 cAGGTGCAGCTGgTGGAGTCTGGGGGAGGCTT 11*06 GGTCAAGCCTGGAGGGTCCCTGAGACTCTCC Native 287 (q V Q L v E S) 41.1 VH VL 124 (D I Q M T Q S P) pCB-IgG-  54 GACATCCAGATGACCCAGTCTCC VK1a CBTAU41.1 126 GACATCCAGATGACCCAGTCTCCAGACTCCCT VL GGCTGTGTCTCTGGGCGAGAGGGTCACCATC IGKV4- 262 GACATCgtGATGACCCAGTCTCCAGACTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGTCACCATC Native 288 (D I v M T Q S P) 41.1 VL CBTAU41.2 VH 127 (E V Q L V Q S) pCB-IgG-  43 GAGGTGCAGCTGGTGCAGTC VH3b CBTAU41.2 129 GAGGTGCAGCTGGTGCAGTCTGGGGGAGGCTT VH GGTCAAGCCTGGAGGGTCCCTGAGACTCTCC IGHV3- 226 cAGGTGCAGCTGGTGgAGTCTGGGGGAGGCTT 11*06 GGTCAAGCCTGGAGGGTCCCTGAGACTCTCC Native 289 (q V Q L v E S) 41.2 VH VL 128 (A I Q L T Q S P) pCB-IgG-  56 GCCATCCAGTTGACCCAGTCTCC VK1c CBTAU41.2 130 GCCATCCAGTTGACCCAGTCTCCAGACTCCCT VL GGCTGTGTCTCTGGGCGAGAGGGTCACCATC IGKV4- 262 gaCATCgtGaTGACCCAGTCTCCAGACTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGTCACCATC Native 290 (d I v m T Q S P) 41.2 VL CBTAU42.1 VH 131 (Q L V Q S E G) pCB-IgG-  36 CAGCTGGTGCAGTC VH1a-c CBTAU42.1 133 CAGCTGGTGCAGTCTGAGGGAGGCCTGGCAGA VH GCCTGGGGGGTCCCTTAGACTC IGHV3- 291 CAGCTGGTGgAGTCTGgGGGAGGCCTGGCAGA 15*01 GCCTGGGGGGTCCCTTAGACTC Native 292 (Q L V e S g g) 42.1 VH VL 132 (E I V L T Q S P) pCB-IgG-  58 GAAATTGTGTTGACGCAGTCTCCAG VK3a CBTAU41.1 134 GAAATTGTGTTGACGCAGTCTCCAGACTCCCT VL GGCTGTGTCTCTGGGCGAGAGGGTCACCATC IGKV4- 262 GAcATcGTGaTGACcCAGTCTCCAGACTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGTCACCATC Native 293 (d I V m T Q S P) 42.1 VL CBTAU43.1 VH 135 (Q V Q L V Q S) pCB-IgG-  36 CAGGTGCAGCTGGTGCAGTC VH1a CBTAU43.1 137 CAGGTGCAGCTGGTGCAGTCTGGAGGAGAGGT GAAAAAGCCGGGGGAGTCTCTGAAGATCTCC IGHV5- 294 gAGGTGCAGCTGGTGCAGTCTGGAGGAGAGGT 51*03 GAAAAAGCCGGGGGAGTCTCTGAAGATCTCC Native 295 (e V Q L V Q S) 43.1 VH VL 136 (E I V L T Q S P) pCB-IgG-  59 GAAATTGTGTTGACACAGTCTCCAG VK3b CBTAU43.1 138 GAAATTGTGTTGACACAGTCTCCAGCCTCCCT VL GGCTGTGTCTCTGGGCGAGAGGGCCACCATC IGKV4- 262 GAcATcGTGaTGACcCAGTCTCCAGCCTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGCCACCATC Native 296 (d I V m T Q S P) 43.1 VL CBTAU44.1 VH 139 (E V Q L V E S) pCB-IgG-  44 GAGGTGCAGCTGGTGGAGTC VH3c CBTAU44.1 141 GAGGTGCAGCTGGTGGAGTCTGGGGGAGGCTT VH GGTACAGCCTGGGGGGTCCCTGAGACTCTCC IGHV3- 297 GAGGTGCAGCTGGTGGAGTCTGGGGGAGGCTT 48*01 GGTACAGCCTGGGGGGTCCCTGAGACTCTCC Native 298 (E V Q L V E S) 44.1 VH VL 140 (D I Q M T Q S) pCB-IgG-  54 GACATCCAGATGACCCAGTCTCC VK1a CBTAU44.1 142 GACATCCAGATGACCCAGTCTCCAGGCACCCT VL GTCTTTGTCTCCAGGGGAAAGAGCCACCCTC IG KV3- 299 GAaATtgtGtTGACgCAGTCTCCAGGCACCCT 20*01 GTCTTTGTCTCCAGGGGAAAGAGCCACCCTC Native 300 (e I v L T Q S) 44.1 VL CBTAU45.1 VH 143 (E V Q L V E S) pCB-IgG-  44 GAGGTGCAGCTGGTGGAGTC VH3c CBTAU45.1 145 GAAATTGTGTTGACACAGTCTCCACTCTCCCT VH GCCCGCCACCCTTGGACAGCCGGCCTCCATC IGHV3- 301 GAGGTGCAGCTGGTGGAGTCTGGGGGAGACTT 15*02 GGTAAAGCCTGGGGGGTCCCTTAGACTCTCC Native 302 (E V Q L V E S) 45.1 VH VL 144 (E I V L T Q S P) pCB-IgG-  59 GAAATTGTGTTGACACAGTCTCCAG VK3b CBTAU45.1 146 GAAATTGTGTTGACACAGTCTCCACTCTCCCT VL GCCCGCCACCCTTGGACAGCCGGCCTCCATC IGKV2- 303 GAtgTTGTGaTGACtCAGTCTCCACTCTCCCT 30*01 GCCCGCCACCCTTGGACAGCCGGCCTCCATC Native 304 (d v V m T Q S P) 45.1 VL CBTAU46.1 VH 147 (Q V Q L V E S) pCB-IgG-  45 CAGGTACAGCTGGTGGAGTCTG VH3d CBTAU46.1 149 CAGGTACAGCTGGTGGAGTCTGGGGGAGGCTT VH GGTACAGCCTGGAGAGTCCCTGAGACTCTCC IGHV3- 305 gAGGTgCAGCTGGTGGAGTCTGGGGGAGGCTT 48*03 GGTACAGCCTGGAGAGTCCCTGAGACTCTCC Native 306 (E V Q L V E S) 46.1 VH VL 148 (D I Q L T Q S P) pCB-IgG-  55 GACATCCAGTTGACCCAGTCTCC VK1b CBTAU46.1 150 GACATCCAGTTGACCCAGTCTCCAGACTCCCT VL GGCTGTGTCTCTGGGCGAGAGGGCCACCATC IGKV4- 262 GACATCgtGaTGACCCAGTCTCCAGACTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGCCACCATC Native 307 (D I v m T Q S P) 46.1 VL CBTAU47.1 VH 151 (Q V Q L V Q S) pCB-IgG-  36 CAGGTGCAGCTGGTGCAGTC VH1a CBTAU47.1 153 CAGGTGCAGCTGGTGCAGTCTGGAGCAGTGGT VH GAAAAAGCCCGGGGAGTCTCTGAAGATCTC IGHV5- 308 gAGGTGCAGCTGGTGCAGTCTGGAGCAGTGGT 51*01 GAAAAAGCCCGGGGAGTCTCTGAAGATCTC Native 309 (E V Q L V Q S) 47.1 VH VL 152 (A I Q L T Q S P) pCB-IgG-  56 GCCATCCAGTTGACCCAGTCTCC VK1c CBTAU44.1 154 GCCATCCAGTTGACCCAGTCTCCAGACTCCCT VL GGCTGTGTCTCTGGGCGAGAGGGCCACCATC IGKV4- 262 GaCATCgtGaTGACCCAGTCTCCAGACTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGCCACCATC Native 310 (d I v m T Q S P) 47.1 VL CBTAU47.2 VH 155 (Q V Q L V E S) pCB-IgG-  45 CAGGTACAGCTGGTGGAGTCTG VH3d CBTAU47.1 157 CAGGTACAGCTGGTGGAGTCTGGAGCAGAACT VH GAAAAAGCCCGGGGAGTCTCTGAAGATCTCC IGHV5- 281 gAGGTgCAGCTGGTGcAGTCTGGAGCAGAACT 51*01 GAAAAAGCCCGGGGAGTCTCTGAAGATCTCC Native 311 (e V Q L V q S) 47.2 VH VL 156 (E I V M T Q S P) pCB-IgG-  60 GAAATAGTGATGACGCAGTCTCCAG VK3c CBTAU44.1 158 GAAATTGTGATGACCCAGTCTCCAGAGTCCCT VL GGCTGTGTCTCTGGGCGAGAGGGCCACCATC IGKV4- 262 GAcATcGTGATGACCCAGTCTCCAGAGTCCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGCCACCATC Native 312 (d I V M T Q S P) 47.2 VL CBTAU49.1 VH 159 (Q V Q L V Q S) pCB-IgG-  36 CAGGTGCAGCTGGTGCAGTC VH1a CBTAU49.1 161 CAGGTGCAGCTGGTGCAGTCTGGGGCAGAGGT VH GAAAAAGCCGTGGGAGTCTCTGAAGATCTCC IGHV5- 294 gAGGTGCAGCTGGTGCAGTCTGGGGCAGAGGT 51*03 GAAAAAGCCGTGGGAGTCTCTGAAGATCTCC Native 313 (e V Q L V Q S) 49.1 VH VL 160 (E I V L T Q S P) pCB-IgG-  63 GAAATTGTGCTGACTCAGTCTCCAG VK6 CBTAU49.1 162 GAAATTGTGCTGACTCAGTCTCCAGACTTCCT VL GGCTGTGTCTCTGGGCGAGAGGGCCACCATC IGKV4- 262 GAcATcGTGaTGACcCAGTCTCCAGACTTCCT 1*01 GGCTGTGTCTCTGGGCGAGAGGGCCACCATC Native 314 (d I V m T Q S P) 49.1 VL

Transfected IgG1 supernatants were assayed for reactivity to tau peptides by ELISA. First, 96 half-well ELISA plates (Costar) were coated with 50 μl of bovine actin (1 μg/ml, Sigma) as a negative control and Affinipure goat anti-human F(ab)2 (2 μg/ml, Jackson Immunoresearch) to confirm antibody production. Plates were coated in TBS overnight at 4° C. The following day, plates were washed five times with TBS/0.05% TWEEN® (TBS-T) and blocked with 150 μl of TBS-T plus 2.5% BSA (blocking buffer) for 2 hour. Tau peptides were captured on streptavidin-coated plates (Pierce) at a concentration of 0.43 μM in 100 μl of TBS. Tau peptides used to set up ELISA assays were the same used as baits in corresponding sorting experiment. Tau peptide-coated plates were then incubated at RT for 1.5 hours. All plates were then washed five times with TBS/0.05% TWEEN® and blocked with 150 μl and 300 μl (tau peptide plates only) of blocking buffer and incubated at RT for 2 hours. IgG transfection supernatants were diluted to 5 μg/ml (based on quantitation by Octet Red) and titrated five-fold in TBS/0.25% BSA. Mouse anti-actin (Sigma, Cat. No. A3853) was used at 1.25 μg/ml as a positive control for bovine actin-coated plates. Commercial grade antibodies were used at 1 μg/ml as positive controls for ELISA assays, including AT8 monoclonal antibody (Thermo, MN1020), AT100 monoclonal antibody (Thermo, MN1060) and AT180 monoclonal antibody (Thermo, MN1040). Primary antibodies were incubated for 2 hours at RT and washed five times in TBS-T. Finally, goat-anti human IgG Fab or goat anti-mouse HRP (Jackson Labs) was used at 1:2000 and 1:4000, respectively, and incubated for 1 hour at RT. Plates were washed five times in TBS-T and developed with SureBlue Reserve TMB Microwell Peroxidase Substrate (KPL). The reaction was halted by the addition of 50 μl and 100 μl (peptide plates) of TMB Stop Solution (KPL) and the absorbance at 450 nm was measured using an ELISA plate reader. Supernatants with the aforementioned binding activities were subsequently reconfirmed in an independent ELISA experiment. Once reconfirmed, a clone was selected for downstream IgG expression and purification (Example 5).

Example 5

IgG1 Expression and Purification of Cloned Anti-Tau Chimeric mAbs

After ELISA screening and confirmation of antibody reactivity, selected clones were expressed as IgG1 s as indicated in Example 4. Cell culture media was harvested and centrifuged to remove the cells after a minimum of 72 hours and up to a maximum of 168 hours. Clarified supernatants were subsequently passed twice through a Protein A Sepharose column (GE Healthcare Life Sciences) and washed with 50 ml of PBS. IgGs were subsequently eluted with 10 ml of IgG elution buffer (Pierce) and neutralized with Tris pH 8.0 and subsequently dialyzed overnight against PBS. Dialyzed samples were concentrated using a 10,000 MWCO ultra-centrifugal unit (Amicon) to a final volume of about 1 mL, and antibody concentrations were determined with Protein A sensor tips using a human IgG standard on the Octet Red384 (ForteBio). Purified antibodies were further quality controlled by performing SDS-PAGE under non-reducing and reducing conditions and by size exclusion chromatography.

Example 6 IgG Binding Reactivity to Tau Peptides

IgG1 s generated and quality controlled as described above were tested by ELISA for their ability to bind to specified cognate peptide(s), as well as non-cognate peptide (Table 10). 96-well ELISA plates (Costar) or streptavidin-coated plates (Pierce) were coated with antigen (bovine actin and affinipure goat anti-human F(ab)2) or tau peptides, respectively, as detailed in Example 4. Purified anti-tau IgGs were diluted to 5 μg/ml in TBS containing 0.25% BSA, and titrated five-fold. Antibody controls and secondary antibodies were used as detailed in Example 4. antibody reactivity at 1 μg/mL was determined by ELISA and scored as no binding (−), weak (−/+), moderate (+), or strong (++). (−) for average of two O.D. 450 nm readings <0.3; (−/+) for >0.5 and <1.0; (+) for >1.0 and <1.5; (++) for >1.5.

TABLE 10 Cognate and non-cognate peptides used  in ELISAs Peptide sequence (px) SEQ denotes phosphorylated ID  Re- mAb Peptide amino acid NO: sults CBTAU- ptau  RSGYSSPG(pS)PG(pT)PGSRSRT 315 + 7.1 194-212 (pS202,  pT205) tau  RSGYSSPGSPGTPGSRSRT 316 − 194-212 CBTAU- ptau  RSGYSSPG(pS)PG(pT)PGSRSRT 315 −/+ 8.1 194-212 (pS202,  pT205) tau  RSGYSSPGSPGTPGSRSRT 316 − 194-212 CBTAU- ptau  GTPGSRSR(pT)P(pS)LPTPPTR 317 ++ 16.1 204-221 (pT212,  pS214) tau  GTPGSRSRTPSLPTPPTR 318 ++ 204-221 CBTAU- ptau  PGSPGTPGSR(pS)RTPSLPT 319 −/+ 18.1 200-217 (pS210) tau  PGSPGTPGSRSRTPSLPT 320 − 200-217 tau  GEPPKSGDRSGYSSPGSPGTPGSRS 321 − 186-253 RTPSLPTPPTREPKKVAVVRTPPKSP SSAKSRLQTAPVPMPDL CBTAU- ptau  EPGSETSDAK(pS)(pT)PTAEDVT 322 ++ 20.1 58-76 (pS68,  pT69) ptau  PGSETSDAKS(pT)P(pT)AEDVTAP 323 ++ 59-78 (pT69,  pT71) ptau  SETSDAKSTP(pT)AEDVTAP 324 −/+ 61-78 (pT71) tau  GLKESPLQTPTEDGSEEPGSETSDA 325 − 42-103 KSTPTAEDVTAPLVDEGAPGKQAA AQPHTEIPEGTTA CBTAU- ptau  RHLSNVSSTG(pS)IDMVD(pS)PQLA 326 ++ 22.1 406-429 TLA (pS416,  pS422) tau  GAEIVYKSPVVSGDTSPRHLSNVSS 327 − 389-441 TGSIDMVDSPQLATLADEVSASLAK QGL CBTAU- ptau  REPKKVAVVR(pT)PPKSPS(pS)AKSR 328 ++ 24.1 221-245 LQT (pT231,  pS238) ptau  VVRTPPKSPS(pS)AKSRLQT 329 ++ 228-245 (pS238) ptau  KVAVVRTPPK(pS)PS(pS)AKSRLQT 330 ++ 225-245 (pS235,  pS238) tau  GEPPKSGDRSGYSSPGSPGTPGSRS 321 ++ 186-253 RTPSLPTPPTREPKKVAVVRTPPKSP SSAKSRLQTAPVPMPDL CBTAU- tau  HVPGGGSVQIVYKPVDLSKVTSKC 331 + 27.1 299-369 GSLGNIHHKPGGGQVEVKSEKLD FKDRVQSKIGSLDNITHVPGGGNK ptau  RSGYSSPG(pS)PG(pT)PGSRSRT 315 − 194-212 (pS202,  pT205) CBTAU- tau  GLKESPLQTPTEDGSEEPGSETSDA 325 ++ 28.1 42-103 KSTPTAEDVTAPLVDEGAPGKQAA AQPHTEIPEGTTA ptau  KSKIG(pS)TENLKHQPGG 332 − 257-272 CBTAU- ptau  RHLSNVSSTG(pS)IDMVD(pS)PQLA 326 + 41.1 406-429 TLA (p416,  p422) tau  GAEIVYKSPVVSGDTSPRHLSNVSS 327 − 389-441 TGSIDMVDSPQLATLADEVSASLAK QGL CBTAU- ptau  RHLSNVSSTG(pS)IDMVD(pS)PQLA 326 + 41.2 406-429 TLA (p416,  p422) tau  GAEIVYKSPVVSGDTSPRHLSNVSS 327 − 389-441 TGSIDMVDSPQLATLADEVSASLAK QGL CBTAU- ptau  RHLSNVSSTG(pS)IDMVD(pS)PQLA 326 ++ 42.1 406-429 TLA (p416,  p422) tau  GAEIVYKSPVVSGDTSPRHLSNVSS 327 − 389-441 TGSIDMVDSPQLATLADEVSASLAK QGL CBTAU- tau  HVPGGGSVQIVYKPVDLSKVTSKC 331 + 43.1 299-369 GSLGNIHHKPGGGQVEVKSEKLD FKDRVQSKIGSLDNITHVPGGGNK ptau  RSGYSSPG(pS)PG(pT)PGSRSRT 315 − 194-212 (pS202,  pT205) CBTAU- ptau  RHLSNVSSTG(pS)IDMVD(pS)PQLA 326 −/+ 44.1 406-429 TLA (p416,  p422) tau  GAEIVYKSPVVSGDTSPRHLSNVSS 327 − 389-441 TGSIDMVDSPQLATLADEVSASLAK QGL CBTAU- ptau  RHLSNVSSTG(pS)IDMVD(pS)PQLA 326 ++ 45.1 406-429 TLA (p416,  p422) tau  GAEIVYKSPVVSGDTSPRHLSNVSS 327 − 389-441 TGSIDMVDSPQLATLADEVSASLAK QGL CBTAU- tau  GLKESPLQTPTEDGSEEPGSETSDA 325 + 46.1 42-103 KSTPTAEDVTAPLVDEGAPGKQAA AQPHTEIPEGTTA ptau  KKVAVVR(pT)PPK(pS)PSSAKS 333 − 224-241 (pT231,  pS235) CBTAU- tau  GLKESPLQTPTEDGSEEPGSETSDA 325 ++ 47.1 42-103 KSTPTAEDVTAPLVDEGAPGKQAA AQPHTEIPEGTTA ptau  KSKIG(pS)TENLKHQPGG 332 − 257-272 (pS262) CBTAU- tau  GLKESPLQTPTEDGSEEPGSETSDA 325 ++ 47.2 42-103 KSTPTAEDVTAPLVDEGAPGKQAA AQPHTEIPEGTTA ptau  KSKIG(pS)TENLKHQPGG 332 − 257-272 (pS262) CBTAU- tau  GLKESPLQTPTEDGSEEPGSETSDA 325 ++ 49.1 42-103 KSTPTAE DVTAPLVDEGAPGKQAAAQPHTE IPEGTTA ptau  KKVAVVR(pT)PPK(pS)PSSAKS 333 − 224-241 (pT231,  pS235) AT8 ptau  RSGYSSPG(pS)PG(pT)PGSRSRT 315 ++ 194-212 (pS202,  pT205) tau  RSGYSSPGSPGTPGSRSRT 316 − 194-212 *Amino acid region on human tau441 isoform

Results are shown in FIGS. 1A-1T. The anti-tau mAbs described herein can be classified into two main groups: those that react only to phosphorylated peptides (phospho-dependent mAbs) and those that react to both phosphorylated and non-phosphorylated peptides (phospho-independent mAbs). Anti-tau mAbs CBTAU-7.1, CBTAU-8.1, CBTAU-18.1, and CBTAU-22.1 were recovered from non-AD individuals using the approach detailed in Example 3. These mAbs are phospho-dependent and, as shown by ELISA (FIGS. 1A-1T), react only with the phosphorylated peptide but not to either a non-phosphorylated peptide spanning that region or a non-phosphorylated version of the peptide. Anti-tau mAbs CBTAU-7.1 and CBTAU-8.1 react specifically to a phosphorylated peptide containing the AT8-binding epitope. This peptide spans amino acids 194 to 212 and contains phosphorylated residues at positions 202 and 205. CBTAU-18.1 reacts to a phosphorylated peptide spanning amino acids 200-217 with a phosphorylated serine residue at position 210. Lastly, CBTAU-22.1 reacts to a peptide spanning amino acids 406-429, with two phosphorylated serines at positions 416 and 422.

Similarly, CBTAU-20.1 was identified from a non-AD individual and is predominately phospho-dependent as it reacts to three different phosphorylated peptides spanning amino acids 59-77. Two of these peptides are dually phosphorylated, one at positions 68 and 69, and the second at positions 69 and 71. CBTAU-20.1 also reacts to a third peptide that is singly phosphorylated at position 71, suggesting that phosphorylation at threonine 71 is sufficient and important for CBTAU-20.1 reactivity. CBTAU-20.1 shows weak reactivity to a non-phosphorylated peptide spanning region 42-103.

Like the aforementioned mAbs, CBTAU-16.1 and CBTAU-24.1 were also recovered from non-AD individuals; however, both mAbs are phospho-independent and, as observed by ELISA, react to both a phosphorylated and non-phosphorylated peptide spanning the specified region. CBTAU-16.1 reacts to amino acid region 204-221, whereas CABTAU-24.1 reacts to three different peptides spanning amino acids 221-245. In addition, two additional anti-tau mAbs (CBTAU-27.1 and CBTAU-28.1) were identified from screens conducted with non-AD donor samples using 60-70 amino acid-length non-phosphorylated peptides corresponding to amino acid regions 42-103 and 299-369, respectively; therefore, both mAbs are specific to non-phosphorylated-tau.

Finally, CBTAU mAbs 41.1, 41.2, 42.1, 43.1, 44.1, 45.1, 46.1, 47.1, 47.2, and 49.1 were identified from a small study where 25 young non-AD (18-27 y.o.), 25 non-AD (55+y.o.), and 25 AD (55+y.o.) individuals were screened. The peptide set that was used for this study included eight phosphorylated peptides (including CBTAU-22.1 cognate peptide) and two non-phosphorylated peptides (CBTAU-27.1 and CBTAU-28.1 cognate peptides). CBTAU mAbs 41.1, 41.2, and 42.1 were recovered from AD donors and react with the CBTAU-22.1 cognate peptide. Similar to CBTAU-22.1, these mAbs are phospho-dependent as shown in FIGS. 1J-1L. Two additional mAbs (CBTAU-44.1 and CBTAU-45.1) were identified from non-AD (55+y.o.) individuals with reactivity to the CBTAU-22.1 cognate peptide. As expected, these two were also phospho-dependent (FIGS. 1N and 10). CBTAU-43.1 was also identified from screens conducted in non-AD (55+y.o.) individuals; however, the mAb was recovered with the CBTAU-27.1 cognate peptide and is specific to non-phosphorylated-tau (FIG. 1M). Lastly, CBTAU-46.1, 47.1, 47.2, and 49.1 were recovered from non-AD (18-27 y.o.) individuals with reactivity to the CBTAU-28.1 peptide and, similar to CBTAU-28.1, are specific to non-phosphorylated-tau (FIGS. 1P-1S).

Example 7 Reactivity to Paired Helical Filaments and Recombinant Tau by ELISA

To further characterize the specificity of some of the chimeric antibodies, their reactivity to recombinant tau, enriched and immunopurified paired helical filaments was tested by ELISA.

PHF-tau was immunopurified according to the protocol of Greenberg and Davies. Briefly, cortical tissues corresponding to Alzheimer's disease individuals were homogenized with 10 volumes of cold buffer (10 mM Tris, pH 7.4, 1 mM EGTA, 0.8 M NaCl and 10% sucrose) and centrifuged at 27,200×g for 20 minutes at 4° C. N-lauroylsarcosine and 2-mercaptoethanol were added to the supernatant to reach a final concentration of 1% (wt/vol) and 1% (vol/vol), respectively. The mixture was incubated at 37° C. for 2-2.5 hours with constant rocking, followed by centrifugation at 108,000×g for 30 minutes at room temperature. The pellet containing PHF-tau was washed three times with PBS and dissolved in PBS without protein inhibitors and further centrifuged at 12,000×g for 5 minutes. The recovered supernatant containing enriched PHF-tau (ePHF-tau) was immunoaffinity purified over an hTau10 affinity column and eluted with 3M or 4 M KSCN overnight at 4° C., followed by dialysis against 1 L PBS at 4° C. with three changes of buffer. hTau10 is an antibody generated in house by immunizing with recombinant tau. It binds to both recombinant and PHF-tau at an amino-terminal epitope. The immunopurified PHF-tau (iPHF-tau) was concentrated with a Sartorius centrifugal filtering device.

For the ELISA, half-area 96-well binding plates (Costar) were coated with 50 μl of antigen in TBS (2 μg/ml recombinant tau, 2 μg/ml bovine action affinipure goat anti-human F(ab)2, 1 μg/ml of affinity-purified paired helical filaments, and 1 μg/ml of monoclonal anti-tau antibody, HT7 (Thermo Scientific, MN1000). The next day, plates were washed with TBS-T and subsequently blocked with 150 μl of TBS plus 2.5% BSA for 2 hours at RT. Following blocking, ePHF-tau was captured for 2 hours at RT on the anti-tau antibody-coated plate. Purified anti-tau IgGs were diluted to 10 μg/ml in TBS plus 0.25% BSA, and IgGs were titrated five-fold at RT for 2 hours. AT8 (10 μg/ml) was used as a positive control for iPHF-tau and captured ePHF-tau. Plates were washed five times with TBS-T and secondary antibodies, diluted in TBS plus 0.25% BSA, were added and incubated at RT for 1 hour. Goat Anti-Human IgG F(ab′)2 (Jackson Labs) was used at a 1:2000 dilution and goat anti-mouse HRP (Jackson Labs) was used at 1:4000 (used for anti-actin control). Following incubation, plates were washed four times in TBS-T and developed with SureBlue Reserve TMB Microwell Peroxidase Substrate (KPL) for approximately 2 minutes. The reaction was immediately halted by the addition of TMB Stop Solution (KPL) and the absorbance at 450 nm was measured using an ELISA plate reader.

Results are shown in FIGS. 2A-2J. As expected, phospho-dependent mAbs CBTAU-7.1, CBTAU-8.1, and CBTAU-18.1 do not react to recombinant tau by ELISA (FIGS. 2A, 2B, and 2D). CBTAU-20.1 shows minor reactivity to recombinant tau consistent with its weak reactivity to a non-phosphorylated peptide spanning region 42-103. Interestingly, these phospho-dependent mAbs do not show any reactivity to paired helical filaments (i.e., ePHF-tau and iPHF-tau) with the exception of CBTAU-7.1, which shows minor reactivity to ePHF-tau at higher antibody concentrations. Lastly, phospho-dependent CBTAU-22.1 shows no reactivity to recombinant tau, but does react to both iPHF-tau and ePHF-tau (FIG. 2F).

Phospho-independent anti-tau mAbs, CBTAU-16.1 and CBTAU-24.1 react to both recombinant tau and both formats of paired helical filaments (i.e., iPHF-tau and ePHF-tau; FIGS. 2C and 2G). CBTAU-28.1 shows strong binding to recombinant tau, with weak immunoreactivity to both PHF-tau formats (FIG. 21). Finally, CBTAU-27.1 shows weak immunoreactivity to both recombinant tau and PHF-tau (FIG. 1H).

Example 8 Reactivity to Paired Helical Filaments and Recombinant Tau by Western Blot Analysis

To extend the observations of the rTau- and PHF-binding ELISAs and to examine if secondary structure plays a role in reactivity, recombinant tau, enriched and immunopurified paired helical filaments were tested by Western blot analysis. Approximately 0.5 μg of iPHF, ePHF, and 1 μg of rTau at a final concentration of 1× NuPAGE® LDS Sample buffer (0.5% LDS final) (Novex, NP0007) was heated at 70° C. for 10 minutes. Samples were loaded onto a 26-well, 4-12% Bis-Tris NOVEX® NuPAGE® gel (Invitrogen) with MOPS SDS running buffer (Novagen, NP0001), and subsequently transferred onto a nitrocellulose membrane. Membrane was blocked overnight in 1×Tris Buffered Saline (TBS) with 0.05% TWEEN®-20 and 4% non-fat dry milk. CBTAU mAbs were used as primary at 25 μg/mL in 1×TBS with 0.05% TWEEN®-20 and 4% non-fat dry milk and incubated for 2 hours at room temperature. The membrane was then washed three times for 5 minutes each in 1×TBS with 0.05% TWEEN®-20. Peroxidase AffiniPure goat anti-human IgG, Fcγ fragment specific (Jackson ImmunoResearch) was then used as secondary at a 1:2000 dilution in 1×TBS with 0.05% TWEEN®-20 and 4% non-fat dry milk and incubated for 45 minutes at RT. The membrane was washed three times for 5 minutes each and developed using the SUPERSIGNAL® West Pico kit (Pierce).

The results for the Western blot analysis are shown in FIG. 3. FIG. 3 shows reactivity of three control antibodies, AT8, AT100, and HT7 (two phospho-tau-specific and total tau-specific, respectively). Both AT8 and AT100 show the triple bands characteristic of PHF-tau, which correspond to approximately 68, 64, and 60 kDa. Contrary to the ELISA results, phospho-dependent mAbs, CBTAU-7.1 and CBTAU-18.1 react to both iPHF-tau and ePHF-tau by Western blot, suggesting that the epitopes for these mAbs are not accessible when tau adopts higher order conformations present in PHF-tau. However, these epitopes become accessible under the strong denaturing conditions of SDS-PAGE. CBTAU-27.1 shows binding to recombinant tau and PHF by Western blot yet weak reactivity to each by ELISA, suggesting that the epitope for this antibody is only exposed under strong denaturing conditions. CBTAU-28.1 reacts strongly to recombinant tau by both Western blot and ELISA, and also shows reactivity to PHF-tau by both assays. CBTAU-28.1 reacts to the E1/E2 region of tau (amino acids 42-103), which is not present in all tau isoforms; therefore, only the 68 and 64 kDa bands on PHF-tau are detected by CBTAU-28.1. Finally, CBTAU-22.1 and CBTAU-24.1 show similar results to the ELISA assay, reacting to either PHF-tau but not recombinant tau and to both PHF-tau and recombinant tau, respectively.

Example 9 Reactivity to Tau Fragment Peptides by ELISA

To characterize the specificity of the recovered antibodies, their reactivity to tau phosphorylated and non-phosphorylated peptides (Tables 11-21, FIGS. 4A-4G) was tested by ELISA. Biotinylated tau peptides were synthesized commercially and dissolved in water at 1 mg/ml and frozen at −80° C. Briefly, 96-well streptavidin-binding plates (Thermo-Fisher) were coated with 2 μg/ml of tau peptides diluted in TBS and incubated overnight at 4° C. The following day, plates were washed with TBS-T and subsequently blocked with 2.5% BSA in TBS for 2 hours at RT. Following blocking, purified anti-tau IgGs were diluted to 2 μg/ml (or to 5 μg/ml and titrated five-fold for finer mapping of CBTAU-27.1, 28.1, 43.1, 46.1, 47.1, 47.2, and 49.1 using peptide sequences in Tables 15-20) in TBS plus 0.25% BSA and incubated at RT for 2 hours. The human-chimerized version of AT8 IgG (at 2 μg/ml) described in Example 11 was used as a positive control in each of the mapping experiments. Plates were washed five times with TBS-T followed by the addition of secondary antibody [goat Anti-Human IgG F(ab′)2 (Jackson Labs) at 1:2000 dilution], diluted in TBS plus 0.25% BSA, and incubated at RT for 1 hour. Following incubation, plates were washed four times in TBS-T and developed with SureBlue Reserve TMB Microwell Peroxidase Substrate (KPL) for approximately 90 seconds. The reaction was immediately halted by the addition of TMB Stop Solution (KPL) and the absorbance at 450 nm was measured using an ELISA plate reader. Each experiment was conducted in triplicate across three different days. Reactivity was considered positive when values were equal to or higher than an OD of 0.4 in the ELISA assay. For determining the reactivity of each mAb to tau-phosphorylated and non-phosphorylated peptides, antibody reactivity at 2 μg/mL was determined by ELISA and scored as no binding (−), weak (−/+), moderate (+), or strong (++). (−) for average of two O.D. 450 nm readings <0.3; (−/+) for >0.5 and <1.0; (+) for >1.0 and <1.5; (++) for >1.5. For finer mapping of CBTAU-27.1, 28.1, 43.1, 46.1, 47.1, 47.2, and 49.1 (detailed on Tables 15-20), antibody reactivity at 1 μg/mL was determined by ELISA and scored as no binding (−), weak (−/+), moderate (+), or strong (++). (−) for average of three O.D. 450 nm readings <0.3; (−/+) for >0.5 and <1.0; (+) for >1.0 and <1.5; (++) for >1.5.

TABLE 11 CBTAU-7.1: Peptides for reactivity by ELISA SEQ Peptide sequence (pX) ID denotes phosphorylated Re- Peptide NO. amino acid sults tau 321 GEPPKSGDRSGYSSPGSPGTPGSR − 186-253 SRTPSLPTPPTREPKKVAVVRTPP KSPSSAKSRLQTAPVPMPDL ptau 334 EPPKSGDRSG(pY)SSPGSPG −/+ 187-212 (pT)PGSRSRT ptau 335 PPKSGDRSGY(pS)SPGSPGT − 188-205 ptau 336 PPKSGDRSGY(pS(pS)PGSPGTP − 188-206 ptau 337 PPKSGDRSGY(pS)SPG(pS) ++ 188-209 PGTPGSR ptau 338 PPKSGDRSGY(pS)SPGSPG(pT) −/+ 188-212 PGSRSRT ptau 339 PKSGDRSGYS(pS)PGSPGTP − 189-206 ptau 340 PKSGDRSGYS(pS)PG(pS) − 189-209 PGTPGSR ptau 341 PKSGDRSGYS(pS)PGSPG(pT) + 189-212 PGSRSRT tau 342 KSGDRSGYSSPGSPGTPGSR − 190-209 ptau 343 GDRSGYSSPG(pS)PGTPGSR − 192-209 ptau 344 GDRSGYSSPG(pS)PG(pT) + 192-212 PGSRSRT ptau 345 GDRSGYSSPG(pS)PGTPG − 192-215 (pS)RSRTPSL ptau 346 GDRSGYSSPG(pS)PGTPGSR − 192-217 (pS)RTPSLPT tau 316 RSGYSSPGSPGTPGSRSRT − 194-212

TABLE 12 CBTAU-18.1: Peptides for reactivity by ELISA SEQ Peptide sequence (pX) ID denotes phosphorylated Re- Peptide NO. amino acid sults ptau 321 GEPPKSGDRSGYSSPGSPGTPGSRSRTPSLPT − 186-253 PPTREPKKVAVVRTPPKSPSSAKSRLQTAPVP MPDL ptau 346 GDRSGYSSPG(pS)PGTPGSR(pS)RTPSLPT ++ 192-217 ptau 315 RSGYSSPG(pS)PG(pT)GSRSRT − 194-212 tau 316 RSGYSSPGSPGTPGSRSRT − 194-212* ptau 347 SGYSSPGSPG(pT)PGSRSRT − 195-212 ptau 348 SGYSSPGSPG(pT)PG(pS)RSRTPSL − 195-215 ptau 349 SGYSSPGSPG(pT)PGSR(pS)RTPSLPT ++ 195-217 ptau 350 SGYSSPGSPG(pT)PGSRSR(pT)PSLPTPP − 195-219 tau 351 SGYSSPGSPGTPGSRSRTPS − 195-214 ptau 352 SSPGSPGTPG(pS)RSRTPSL − 198-215 ptau 353 SPGSPGTPG(pS)R(pS)RTPSLPT ++ 198-217 ptau 354 SSPGSPGTPG(pS)RSR(pT)PSLPTPP −/+ 198-219 ptau 355 SSPGSPGTPG(pS)RSRTP(pS)LPTPPTR − 198-221 tau 356 SSPGSPGTPGSRSRTPSLPT − 198-217 ptau 319 PGSPGTPGSR(pS)RTPSLPT + 200-217 tau 320 PGSPGTPGSRSRTPSLPT − 200-217 ptau 357 PGSPGTPGSR(pS)R(pT)PSLPTPP −/+ 200-219 ptau 358 PGSPGTPGSR(pS)RTP(pS)LPTPPTR − 200-221 ptau 359 PGSPGTPGSR(pS)RTPSLP(pT)PPTREPK − 200-224

table 13 CBTAU-22.1: Peptides for reactivity by ELISA SEQ Peptide sequence (pX) ID denotes phosphorylated Re- Peptide NO. amino acid sults ptau 360 SPRHLSNVSS(pT)GSIDMVD − 404-421 ptau 361 SPRHLSNVSS(pT)GSIDMVD(pS)PQLATLA ++ 404-429 tau 362 PRHLSNVSSTGSIDMVDSP − 405-423 ptau 363 RHLSNVSSTG(pS)IDMVDSP − 406-423 ptau 326 RHLSNVSSTG(pS)IDMVD(pS)PQLATLA ++ 406-429 tau 364 SNVSSTGSIDMVDSPQLATL − 409-428 ptau 365 SSTGSIDMVD(pS)PQLATLA ++ 412-429 ptau 366 SSTGSIDMVD(pS)PQLA(pT)LADEVSA ++ 412-434

TABLE 14 CBTAU-24.1: Peptides for reactivity by ELISA SEQ Peptide sequence (pX) ID denotes phosphorylated Re- Peptide NO. amino acid sults tau 367 GEPPKSGDRSGYSSPGSPGTPGSRSKYP ++ 221-253 SLPTPPTREPKKVAVVRTPPKSPSSAKS RLQTAPVPMPDL ptau 368 REPKKVAVVR(pT)PPKSPSS − 221-238 ptau 369 REPKKVAVVR(pT)PPK(pS)PSSAKSR − 221-242 ptau 370 REPKKVAVVR(pT)PPKSP(pS)SAKSRLQ − 221-244 ptau 328 REPKKVAVVR(pT)PPKSPS(pS)AKSRLQT ++ 221-245 ptau 371 KVAVVRTPPK(pS)PSSAKSR − 225-242 ptau 372 KVAVVRTPPK(pS)P(pS)SAKSRLQ −/+ 225-244 ptau 330 KVAVVRTPPK(pS)PS(pS)AKSRLQT ++ 225-245 ptau 373 AVVRTPPKSP(pS)SAKSRLQ ++ 227-244 ptau 374 AVVRTPPKSP(pS)(pS)AKSRLQT ++ 227-245 ptau 329 VVRTPPKSPS(pS)AKSRLQT ++ 228-245

TABLE 15 CBTAU-27.1: Peptides for reactivity by ELISA SEQ Peptide sequence (pX) ID denotes phosphorylated Re- Peptide NO. amino acid sults Cluster 1 tau 331 HVPGGGSVQIVYKPVDLSKVTSKCGSLGNI ++ 299-369 HHKPGGGQVEVKSEKLDFKDRVQSKIGSLD NITHVPGGGNK Cluster 2 ptau 360 SPRHLSNVSS(pT)GSIDMVD − 404-421 p414 ptau 361 SPRHLSNVSS(pT)GSIDMVD(pS)PQLATLA −/+ 404-429 p414, 422 ptau 363 RHLSNVSSTG(pS)IDMVDSP − 406-423 p416 ptau 326 RHLSNVSSTG(pS)IDMVD(pS)PQLATLA −/+ 406-429 p416, 422 ptau 365 SSTGSIDMVD(pS)PQLATLA −/+ 412-429 p422 ptau 366 SSTGSIDMVD(pS)PQLA(pT)LADEVSA −/+ 412-434 p422, 427 tau 375 HVPGGGSVQIVYKPVDLSKV + 299-318 tau 376 VYKPVDLSKVTSKCGSLGNI −/+ 309-328 tau 377 TSKCGSLGNIHHKPGGGQVE − 319-338 tau 378 HHKPGGGQVEVKSEKLDFKD − 329-348 tau 379 VKSEKLDFKDRVQSKIGSLD − 339-358 tau 380 RVQSKIGSLDNITHVPGGGNK − 349-369

TABLE 16 CBTAU-28.1: Peptides for reactivity by ELISA SEQ ID Re- Peptide NO. Peptide sequence sults tau 325 GLKESPLQTPTEDGSEEPGSETSDAKSTPTAE ++ 42-103 DVTAPLVDEGAPGKQAAAQPHTEIPEGTTA tau 381 GLKESPLQTPTEDGSEEPGS − 42-61 tau 382 TEDGSEEPGSETSDAKSTPT ++ 52-71 ptau 383 EPGSETSDAK(pS)TPTAEDV − 58-75 tau 384 ETSDAKSTPTAEDVTAPLVD − 62-81 tau 385 AEDVTAPLVDEGAPGKQAAA − 72-91 tau 386 EGAPGKQAAAQPHTEIPEGTTA − 82-103

TABLE 17 CBTAU-43.1: Peptides for reactivity by ELISA SEQ ID Re- Peptide NO. Peptide sequence sults tau 331 HVPGGGSVQIVYKPVDLSKVTSKCGSLGN ++ 299-369 IHHKPGGGQVEVKSEKLDFKDRVQSKIGS LDNITHVPGGGNK tau 375 HVPGGGSVQIVYKPVDLSKV ++ 299-318 tau 376 VYKPVDLSKVTSKCGSLGNI ++ 309-328 tau 377 TSKCGSLGNIHHKPGGGQVE − 319-338 tau 378 HHKPGGGQVEVKSEKLDFKD − 329-348 tau 379 VKSEKLDFKDRVQSKIGSLD − 339-358 tau 380 RVQSKIGSLDNITHVPGGGNK − 349-369

TABLE 18 CBTAU-46.1: Peptides for reactivity by ELISA SEQ ID Re- Peptide NO. Peptide sequence sults tau 325 GLKESPLQTPTEDGSEEPGSETSDA ++ 42-103 KSTPTAEDVTAPLVDEGAPGKQAAA QPHTEIPEGTTA tau 381 GLKESPLQTPTEDGSEEPGS − 42-61 tau 382 TEDGSEEPGSETSDAKSTPT − 52-71 tau 384 ETSDAKSTPTAEDVTAPLVD − 62-81 tau 385 AEDVTAPLVDEGAPGKQAAA − 72-91 tau 386 EGAPGKQAAAQPHTEIPEGTTA ++ 82-103

TABLE 19 CBTAU-47.1 and CBTAU-47.2: Peptides for reactivity by ELISA SEQ ID Re- Peptide NO. Peptide sequence sults tau 325 GLKESPLQTPTEDGSEEPGSETSDA ++ 42-103 KSTPTAEDVTAPLVDEGAPGKQAAA QPHTEIPEGTTA tau 381 GLKESPLQTPTEDGSEEPGS − 42-61 tau 382 TEDGSEEPGSETSDAKSTPT ++ 52-71 tau 384 ETSDAKSTPTAEDVTAPLVD − 62-81 tau 385 AEDVTAPLVDEGAPGKQAAA − 72-91 tau 386 EGAPGKQAAAQPHTEIPEGTTA − 82-103

TABLE 20 CBTAU-49.1: Peptides for reactivity by ELISA SEQ ID Re- Peptide NO. Peptide sequence sults tau 325 GLKESPLQTPTEDGSEEPGSETSDA ++ 42-103 KSTPTAEDVTAPLVDEGAPGKQAAA QPHTEIPEGTTA tau 381 GLKESPLQTPTEDGSEEPGS − 42-61 tau 382 TEDGSEEPGSETSDAKSTPT ++ 52-71 tau 384 ETSDAKSTPTAEDVTAPLVD − 62-81 tau 385 AEDVTAPLVDEGAPGKQAAA − 72-91 tau 386 EGAPGKQAAAQPHTEIPEGTTA − 82-103

TABLE 21 AT8 Peptides for reactivity by ELISA SEQ Peptide sequence (pX) ID denotes phosphorylated Re- Peptide NO. amino acid sult ptau 341 PKSGDRSGYS(pS)PGSPG(pT) − 189-212 PGSRSRT tau 387 GDRSGYSSPGSPGTPGSRSR − 192-211 ptau 343 GDRSGYSSPG(pS)PGTPGSR − 192-209 ptau 344 GDRSGYSSPG(pS)PG(pT)PGSRSRT ++ 192-212 ptau 345 GDRSGYSSPG(pS)PGTPG(pS)RSRTPSL − 192-215 ptau 346 GDRSGYSSPG(pS)PGTPGSR(pS) − 192-217 RTPSLPT ptau 315 RSGYSSPG(pS)PG(pT)PGSRSRT ++ 194-212 tau 316 RSGYSSPGSPGTPGSRSRT − 194-212* ptau 347 SGYSSPGSPG(pT)PGSRSRT − 195-212

Although CBTAU-7.1 was recovered using a peptide that contains the AT8 epitope (Table 21; 192-212; pS202, pT205), the phospho-residues contributing to binding for CBTAU-7.1 appeared to be promiscuous involving positions S202+T205, but also combinations of S198+S202, S198+T205, S199+T205 and possibly Y197+T205. Unphosphorylated peptides showed no reactivity to CBTAU-7.1. For CBTAU-18.1, the minimal epitope was found to consist of amino acids 198-217 and dependent on pS210 but not when T212, S214 or T217 were also phosphorylated. CBTAU-22.1 reactivity was found to be dependent on pS422, while antibody CBTAU-24.1 revealed strong binding to its corresponding unphosphorylated peptide and, thus, unaffected by phosphorylation.

CBTAU-27.1 and CBTAU-43.1 were recovered using an unphosphorylated peptide spanning amino acids 299-369. Interestingly, overlapping peptides within this region revealed similar binding requirements for both mAbs (i.e., CBTAU-27.1 and CBTAU-43.1 reacted to peptides spanning amino acids 299-318 and 309-328, respectively), suggesting that the epitope for both mAbs is within regions 299-328 on tau441 (FIGS. 4A and 4C).

CBTAU-28.1, 46.1, 47.1, 47.2, and 49.1 were recovered from human donor samples using a peptide spanning regions 42-103 on tau441. Testing the reactivity of each mAb against a smaller overlapping set of peptides showed similar binding for CBTAU-47.1, 47.2, and 49.1 as CBTAU-28.1 (i.e., reactivity to a peptide spanning regions 52-71), suggesting comparable binding requirements; however, CBTAU-46.1 bound to a region C-terminal to the aforementioned mAbs (i.e., 82-1031; FIGS. 4B and 4D-4G).

Example 10 Alanine Scanning of Peptide Epitopes

To further characterize the specificity and amino acid contribution to binding of each of the recover mAbs, their reactivity to tau peptides with each position replaced with Alanine was tested by ELISA. All experimental protocols were identical to Example 9. Antibody reactivity at 1 μg/mL was determined by ELISA and scored as no binding (−), weak (−/+), moderate (+), or strong (++). (−) for average of two O.D. 450 nm readings <0.3; (−/+) for >0.5 and <1.0; (+) for >1.0 and <1.5; (++) for >1.5. Results for each antibody are shown in Tables 22-29.

TABLE 22 Alanine scanning results for CBTAU-7.1 and CBTAU-8.1 SEQ Peptide sequence (pX) Re- Re- Region ID denotes phosphorylated sults sults (Tau44) NO amino acid 7.1 8.1 ptau 334 EPPKSGDRSGYSSPG(pS)PG(pT) ++ ++ 187-212 PGSRSRT ptau 388 APPKSGDRSGYSSPG(pS)PG(pT) + ++ 187-212 PGSRSRT (A187) ptau 389 EAPKSGDRSGYSSPG(pS)PG(pT) + ++ 187-212 PGSRSRT (A188) ptau 390 EPAKSGDRSGYSSPG(pS)PG(pT) + ++ 187-212 PGSRSRT (A189) ptau 391 EPPASGDRSGYSSPG(pS)PG(pT) ++ ++ 187-212 PGSRSRT (A190) ptau 392 EPPKAGDRSGYSSPG(pS)PG(pT) ++ ++ 187-212 PGSRSRT (A191) ptau 393 EPPKSADRSGYSSPG(pS)PG(pT) ++ ++ 187-212 PGSRSRT (A192) ptau 394 EPPKSGARSGYSSPG(pS)PG(pT) ++ ++ 187-212 PGSRSRT (A193) ptau 395 EPPKSGDASGYSSPG(pS)PG(pT) ++ ++ 187-212 PGSRSRT (A194) ptau 396 EPPKSGDRAGYSSPG(pS)PG(pT) ++ ++ 187-212 PGSRSRT (A195) ptau 397 EPPKSGDRSAYSSPG(pS)PG(pT) ++ ++ 187-212 PGSRSRT (A196) ptau 398 EPPKSGDRSGASSPG(pS)PG(pT) ++ ++ 187-212 PGSRSRT (A197) ptau 399 EPPKSGDRSGYASPG(pS)PG(pT) ++ ++ 187-212 PGSRSRT (A198) ptau 400 EPPKSGDRSGYSAPG(pS)PG(pT) + ++ 187-212 PGSRSRT (A199) ptau 401 EPPKSGDRSGYSSAG(pS)PG(pT) + ++ 187-212 PGSRSRT (A200) ptau 402 EPPKSGDRSGYSSPA(pS)PG(pT) ++ ++ 187-212 PGSRSRT (A201) ptau 403 EPPKSGDRSGYSSPGAPG(pT) + ++ 187-212 PGSRSRT (A202) ptau 404 EPPKSGDRSGYSSPG(pS)AG(pT) ++ ++ 187-212 PGSRSRT (A203) ptau 405 EPPKSGDRSGYSSPG(pS)PA(pT) −/+ + 187-212 PGSRSRT (A204) ptau 406 EPPKSGDRSGYSSPG(pS) −/+ −/+ 187-212 PGAPGSRSRT (A205) ptau 407 EPPKSGDRSGYSSPG(pS)PG(pT) −/+ − 187-212 AGSRSRT (A206) ptau 408 EPPKSGDRSGYSSPG(pS)PG(pT) ++ −/+ 187-212 PASRSRT (A207) ptau 409 EPPKSGDRSGYSSPG(pS)PG(pT) ++ ++ 187-212 PGARSRT (A208) ptau 410 EPPKSGDRSGYSSPG(pS)PG(pT) ++ 187-212 PGSASRT (A209) ptau 411 EPPKSGDRSGYSSPG(pS)PG(pT) ++ ++ 187-212 PGSRART (A210) ptau 412 EPPKSGDRSGYSSPG(pS)PG(pT) ++ ++ 187-212 PGSRSAT (A211) ptau 413 EPPKSGDRSGYSSPG(pS)PG(pT) ++ ++ 187-212 PGSRSRA (A212)

TABLE 23 Alanine scanning results for CBTAU-22.1 SEQ Peptide sequence (pX) Region ID denotes phosphorylated Re- (Tau441) NO amino acid sults ptau 326 RHLSNVSSTG(pS)IDMVD(pS)PQLATLA ++ 406-429 ptau 414 AHLSNVSSTG(pS)IDMVD(pS)PQLATLA ++ 406-429 (A406) ptau 415 RALSNVSSTG(pS)IDMVD(pS)PQLATLA ++ 406-429 (A407) ptau 416 RHASNVSSTG(pS)IDMVD(pS)PQLATLA ++ 406-429 (A408) ptau 417 RHLANVSSTG(pS)IDMVD(pS)PQLATLA ++ 406-429 (A409) ptau 418 RHLSAVSSTG(pS)IDMVD(pS)PQLATLA ++ 406-429 (A410) ptau 419 RHLSNASSTG(pS)IDMVD(pS)PQLATLA ++ 406-429 (A411) ptau 420 RHLSNVASTG(pS)IDMVD(pS)PQLATLA ++ 406-429 (A412) ptau 421 RHLSNVSATG(pS)IDMVD(pS)PQLATLA ++ 406-429 (A413) ptau 422 RHLSNVSSAG(pS)IDMVD(pS)PQLATLA ++ 406-429 (A414) ptau 423 RHLSNVSSTA(pS)IDMVD(pS)PQLATLA ++ 406-429 (A415) ptau 424 RHLSNVSSTGAIDMVD(pS)PQLATLA ++ 406-429 (A416) ptau 425 RHLSNVSSTG(pS)ADMVD(pS)PQLATLA ++ 406-429 (A417) ptau 426 RHLSNVSSTG(pS)IAMVD(pS)PQLATLA ++ 406-429 (A418) ptau 427 RHLSNVSSTG(pS)IDAVD(pS)PQLATLA ++ 406-429 (A419) ptau 428 RHLSNVSSTG(pS)IDMAD(pS)PQLATLA ++ 406-429 (A420) ptau 429 RHLSNVSSTG(pS)IDMVA(pS)PQLATLA −/+ 406-429 (A421) ptau 430 RHLSNVSSTG(pS)IDMVDAPQLATLA − 406-429 (A422) ptau 431 RHLSNVSSTG(pS)IDMVD(pS)AQLATLA ++ 406-429 (A423) ptau 432 RHLSNVSSTG(pS)IDMVD(pS)PALATLA ++ 406-429 (A424) ptau 433 RHLSNVSSTG(pS)IDMVD(pS)PQAATLA ++ 406-429 (A425) ptau 434 RHLSNVSSTG(pS)IDMVD(pS)PQLAALA ++ 406-429 (A427) ptau 435 RHLSNVSSTG(pS)IDMVD(pS)PQLATAA ++ 406-429 (A428)

TABLE 24 CBTAU-24.1 Alanine Scan Results SEQ Peptide sequence (pX) Region ID denotes phosphorylated Re- (Tau441) NO amino acid sults ptau 328 REPKKVAVVR(pT)PPKSPS(pS)AKSRLQT ++ 221-245 ptau 436 RAPKKVAVVR(pT)PPKSPS(pS)AKSRLQT ++ 221-245 (A222) ptau 437 REAKKVAVVR(pT)PPKSPS(pS)AKSRLQT ++ 221-245 (A223) ptau 438 REPAKVAVVR(pT)PPKSPS(pS)AKSRLQT ++ 221-245 (A224) ptau 439 REPKAVAVVR(pT)PPKSPS(pS)AKSRLQT ++ 221-245 (A225) ptau 440 REPKKAAVVR(pT)PPKSPS(pS)AKSRLQT ++ 221-245 (A226) ptau 441 REPKKVAAVR(pT)PPKSPS(pS)AKSRLQT ++ 221-245 (A228) ptau 442 REPKKVAVAR(pT)PPKSPS(pS)AKSRLQT ++ 221-245 (A229) ptau 443 REPKKVAVVA(pT)PPKSPS(pS)AKSRLQT ++ 221-245 (A230) ptau 444 REPKKVAVVRAPPKSPS(pS)AKSRLQT ++ 221-245 (A231) ptau 445 REPKKVAVVR(pT)APKSPS(pS)AKSRLQT ++ 221-245 (A232) ptau 446 REPKKVAVVR(pT)PAKSPS(pS)AKSRLQT ++ 221-245 (A233) ptau 447 REPKKVAVVR(pT)PPASPS(pS)AKSRLQT ++ 221-245 (A234) ptau 448 REPKKVAVVR(pT)PPKAPS(pS)AKSRLQT ++ 221-245 (A235) ptau 449 REPKKVAVVR(pT)PPKSAS(pS)AKSRLQT − 221-245 (A236) ptau 450 REPKKVAVVR(pT)PPKSPA(pS)AKSRLQT ++ 221-245 (A237) ptau 451 REPKKVAVVR(pT)PPKSPSAAKSRLQT ++ 221-245 (A238) ptau 452 REPKKVAVVR(pT)PPKSPS(pS)AASRLQT ++ 221-245 (A240) ptau 453 REPKKVAVVR(pT)PPKSPS(pS)AKARLQT ++ 221-245 (A241) ptau 454 REPKKVAVVR(pT)PPKSPS(pS)AKSALQT ++ 221-245 (A242) ptau 455 REPKKVAVVR(pT)PPKSPS(pS)AKSRAQT ++ 221-245 (A243) ptau 456 REPKKVAVVR(pT)PPKSPS(pS)AKSRLAT ++ 221-245 (A244) ptau 457 REPKKVAVVR(pT)PPKSPS(pS)AKSRLQA ++ 221-245 (A245)

TABLE 25 CBTAU-27.1 Alanine Scan Results SEQ Region ID (Tau441) NO: Peptide sequence Results tau 458 HVPGGGSVQIVYKPVDLSKVTSKCG ++ 299-323 tau 459 AVPGGGSVQIVYKPVDLSKVTSKCG ++ 299-323 (A299) tau 460 HAPGGGSVQIVYKPVDLSKVTSKCG ++ 299-323 (A300) tau 461 HVAGGGSVQIVYKPVDLSKVTSKCG ++ 299-323 (A301) tau 462 HVPAGGSVQIVYKPVDLSKVTSKCG ++ 299-323 (A302) tau 463 HVPGAGSVQIVYKPVDLSKVTSKCG ++ 299-323 (A303) tau 464 HVPGGASVQIVYKPVDLSKVTSKCG ++ 299-323 (A304) tau 465 HVPGGGAVQIVYKPVDLSKVTSKCG ++ 299-323 (A305) tau 466 HVPGGGSAQIVYKPVDLSKVTSKCG ++ 299-323 (A306) tau 467 HVPGGGSVAIVYKPVDLSKVTSKCG ++ 299-323 (A307) tau 468 HVPGGGSVQAVYKPVDLSKVTSKCG ++ 299-323 (A308) tau 469 HVPGGGSVQIAYKPVDLSKVTSKCG ++ 299-323 (A309) tau 470 HVPGGGSVQIVAKPVDLSKVTSKCG ++ 299-323 (A310) tau 471 HVPGGGSVQIVYAPVDLSKVTSKCG ++ 299-323 (A311) tau 472 HVPGGGSVQIVYKAVDLSKVTSKCG ++ 299-323 (A312) tau 473 HVPGGGSVQIVYKPADLSKVTSKCG ++ 299-323 (A313) tau 474 HVPGGGSVQIVYKPVALSKVTSKCG −/+ 299-323 (A314) tau 475 HVPGGGSVQIVYKPVDASKVTSKCG − 299-323 (A315) tau 476 HVPGGGSVQIVYKPVDLAKVTSKCG ++ 299-323 (A316) tau 477 HVPGGGSVQIVYKPVDLSAVTSKCG − 299-323 (A317) tau 478 HVPGGGSVQIVYKPVDLSKATSKCG ++ 299-323 (A318) tau 479 HVPGGGSVQIVYKPVDLSKVASKCG ++ 299-323 (A319) tau 480 HVPGGGSVQIVYKPVDLSKVTAKCG ++ 299-323 (A320) tau 481 HVPGGGSVQIVYKPVDLSKVTSACG ++ 299-323 (A321) tau 482 HVPGGGSVQIVYKPVDLSKVTSKAG ++ 299-323 (A322) tau 483 HVPGGGSVQIVYKPVDLSKVTSKCA ++ 299-323 (A323)

TABLE 26 CBTAU-28.1 Alanine Scan Results SEQ ID Region (Tau441) NO Peptide sequence Results tau 52-71 382 TEDGSEEPGSETSDAKSTPT ++ tau 52-71 (A52) 484 AEDGSEEPGSETSDAKSTPT ++ tau 52-71 (A53) 485 TADGSEEPGSETSDAKSTPT ++ tau 52-71 (A54) 486 TEAGSEEPGSETSDAKSTPT ++ tau 52-71 (A55) 487 TEDASEEPGSETSDAKSTPT ++ tau 52-71 (A56) 488 TEDGAEEPGSETSDAKSTPT ++ tau 52-71 (A57) 489 TEDGSAEPGSETSDAKSTPT ++ tau 52-71 (A58) 490 TEDGSEAPGSETSDAKSTPT ++ tau 52-71 (A59) 491 TEDGSEEAGSETSDAKSTPT −/+ tau 52-71 (A60) 492 TEDGSEEPASETSDAKSTPT ++ tau 52-71 (A61) 493 TEDGSEEPGAETSDAKSTPT ++ tau 52-71 (A62) 494 TEDGSEEPGSATSDAKSTPT − tau 52-71 (A63) 495 TEDGSEEPGSEASDAKSTPT −/+ tau 52-71 (A64) 496 TEDGSEEPGSETADAKSTPT ++ tau 52-71 (A65) 497 TEDGSEEPGSETSAAKSTPT − tau 52-71 (A67) 498 TEDGSEEPGSETSDAASTPT − tau 52-71 (A68) 499 TEDGSEEPGSETSDAKATPT ++ tau 52-71 (A69) 500 TEDGSEEPGSETSDAKSAPT ++ tau 52-71 (A70) 501 TEDGSEEPGSETSDAKSTAT ++ tau 52-71 (A71) 502 TEDGSEEPGSETSDAKSTPA ++

TABLE 27 CBTAU-43.1 Alanine Scan Results SEQ Region ID (Tau441) NO: Peptide sequence Results tau 299-323 458 HVPGGGSVQIVYKPVDLSKVTSKCG ++ tau 299-323 459 AVPGGGSVQIVYKPVDLSKVTSKCG ++ (A299) tau 299-323 460 HAPGGGSVQIVYKPVDLSKVTSKCG ++ (A300) tau 299-323 461 HVAGGGSVQIVYKPVDLSKVTSKCG ++ (A301) tau 299-323 462 HVPAGGSVQIVYKPVDLSKVTSKCG ++ (A302) tau 299-323 463 HVPGAGSVQIVYKPVDLSKVTSKCG ++ (A303) tau 299-323 464 HVPGGASVQIVYKPVDLSKVTSKCG ++ (A304) tau 299-323 465 HVPGGGAVQIVYKPVDLSKVTSKCG ++ (A305) tau 299-323 466 HVPGGGSAQIVYKPVDLSKVTSKCG ++ (A306) tau 299-323 467 HVPGGGSVAIVYKPVDLSKVTSKCG ++ (A307) tau 299-323 468 HVPGGGSVQAVYKPVDLSKVTSKCG ++ (A308) tau 299-323 469 HVPGGGSVQIAYKPVDLSKVTSKCG ++ (A309) tau 299-323 470 HVPGGGSVQIVAKPVDLSKVTSKCG ++ (A310) tau 299-323 471 HVPGGGSVQIVYAPVDLSKVTSKCG ++ (A311) tau 299-323 472 HVPGGGSVQIVYKAVDLSKVTSKCG −/+ (A312) tau 299-323 473 HVPGGGSVQIVYKPADLSKVTSKCG ++ (A313) tau 299-323 474 HVPGGGSVQIVYKPVALSKVTSKCG ++ (A314) tau 299-323 475 HVPGGGSVQIVYKPVDASKVTSKCG − (A315) tau 299-323 476 HVPGGGSVQIVYKPVDLAKVTSKCG ++ (A316) tau 299-323 477 HVPGGGSVQIVYKPVDLSAVTSKCG − (A317) tau 299-323 478 HVPGGGSVQIVYKPVDLSKATSKCG ++ (A318) tau 299-323 479 HVPGGGSVQIVYKPVDLSKVASKCG ++ (A319) tau 299-323 480 HVPGGGSVQIVYKPVDLSKVTAKCG ++ (A320) tau 299-323 481 HVPGGGSVQIVYKPVDLSKVTSACG ++ (A321) tau 299-323 482 HVPGGGSVQIVYKPVDLSKVTSKAG ++ (A322) tau 299-323 483 HVPGGGSVQIVYKPVDLSKVTSKCA ++ (A323)

TABLE 28 CBTAU-47.1 and 47.2 Alanine Scan Results SEQ Region ID CBTAU- CBTAU- (Tau441) NO Peptide sequence 47.1 47.2 tau 52-71 382 TEDGSEEPGSETSDAKSTPT ++ ++ tau 52-71 484 AEDGSEEPGSETSDAKSTPT ++ ++ (A52) tau 52-71 485 TADGSEEPGSETSDAKSTPT ++ ++ (A53) tau 52-71 486 TEAGSEEPGSETSDAKSTPT ++ ++ (A54) tau 52-71 487 TEDASEEPGSETSDAKSTPT ++ ++ (A55) tau 52-71 488 TEDGAEEPGSETSDAKSTPT ++ ++ (A56) tau 52-71 489 TEDGSAEPGSETSDAKSTPT ++ ++ (A57) tau 52-71 490 TEDGSEAPGSETSDAKSTPT ++ ++ (A58) tau 52-71 491 TEDGSEEAGSETSDAKSTPT − − (A59) tau 52-71 492 TEDGSEEPASETSDAKSTPT ++ ++ (A60) tau 52-71 493 TEDGSEEPGAETSDAKSTPT −/+ ++ (A61) tau 52-71 494 TEDGSEEPGSATSDAKSTPT − − (A62) tau 52-71 495 TEDGSEEPGSEASDAKSTPT − − (A63) tau 52-71 496 TEDGSEEPGSETADAKSTPT ++ ++ (A64) tau 52-71 497 TEDGSEEPGSETSAAKSTPT − − (A65) tau 52-71 498 TEDGSEEPGSETSDAASTPT − − (A67) tau 52-71 499 TEDGSEEPGSETSDAKATPT ++ ++ (A68) tau 52-71 500 TEDGSEEPGSETSDAKSAPT ++ ++ (A69) tau 52-71 501 TEDGSEEPGSETSDAKSTAT ++ ++ (A70) tau 52-71 502 TEDGSEEPGSETSDAKSTPA ++ ++ (A71)

TABLE 29 CBTAU-49.1 Alanine Scan Results SEQ Region ID (Tau441) NO Peptide sequence Results tau 52-71 382 TEDGSEEPGSETSDAKSTPT ++ tau 52-71 (A52) 484 AEDGSEEPGSETSDAKSTPT ++ tau 52-71 (A53) 485 TADGSEEPGSETSDAKSTPT ++ tau 52-71 (A54) 486 TEAGSEEPGSETSDAKSTPT ++ tau 52-71 (A55) 487 TEDASEEPGSETSDAKSTPT ++ tau 52-71 (A56) 488 TEDGAEEPGSETSDAKSTPT ++ tau 52-71 (A57) 489 TEDGSAEPGSETSDAKSTPT ++ tau 52-71 (A58) 490 TEDGSEAPGSETSDAKSTPT ++ tau 52-71 (A59) 491 TEDGSEEAGSETSDAKSTPT − tau 52-71 (A60) 492 TEDGSEEPASETSDAKSTPT ++ tau 52-71 (A61) 493 TEDGSEEPGAETSDAKSTPT − tau 52-71 (A62) 494 TEDGSEEPGSATSDAKSTPT − tau 52-71 (A63) 495 TEDGSEEPGSEASDAKSTPT + tau 52-71 (A64) 496 TEDGSEEPGSETADAKSTPT + tau 52-71 (A65) 497 TEDGSEEPGSETSAAKSTPT − tau 52-71 (A67) 498 TEDGSEEPGSETSDAASTPT − tau 52-71 (A68) 499 TEDGSEEPGSETSDAKATPT + tau 52-71 (A69) 500 TEDGSEEPGSETSDAKSAPT + tau 52-71 (A70) 501 TEDGSEEPGSETSDAKSTAT + tau 52-71 (A71) 502 TEDGSEEPGSETSDAKSTPA +

Although CBTAU-7.1 and CBTAU-8.1 were recovered using a tau phosphopeptide containing the AT8 epitope (i.e., pS202, pT205), both mAbs exhibited different epitope requirements according to the alanine scan results (Table 22). In addition to S202 and T205, substitutions at positions G204 and P206 resulted in reduced binding for CBTAU-7.1. In contrast, alanine substitutions at positions G204, T205, P206, and 8209 reduced the reactivity of CBTAU-8.1 to the peptide, yet the S202A substitution had no effect. Like AT8, both mAbs are phospho-dependent, but require additional (non-phosphorylated residues) for binding. The alanine scan results for CBTAU-22.1 showed a dependency on phosphorylation at S422 (Table 23), as substitution at this position completed inhibited binding. Substitution at D421 resulted in a reduction but not a complete inhibition in binding. Finally, alanine scan results for CBTAU-24.1 showed P236 to be the only critical residue for binding (Table 24).

To map the critical contact residues for CBTAU-27.1 and 43.1, alanine scanning was also conducted within regions 299-323 of tau (Table 25 and Table 27, respectively). The critical contact residues for CBTAU-27.1 binding were shown to be D314, L315, and K317. The results suggest that residues D314 and K317 may form salt bridge interactions between the epitope and CDR residues on the mAb. While CBTAU-43.1 was recovered using the cognate peptide for CBAU-27.1, the critical residues according to the alanine scan were different. In addition to L315 and K317, the proline at position 312 was shown to be an important contact for CBTAU-43.1 binding. Lastly, alanine scanning was also conducted for CBTAU-28.1 as well as to CBTAU-47.1, 47.1, and 49.1 (Tables 26, 28, 29). As shown in Example 9, CBTAU mAbs 47.1, 47.2, 49.1 mapped to the same peptide region as CBTAU-28.1 (i.e., 52-71). Interestingly, all mAbs shared identical binding requirements as to CBTAU-28.1. The critical contact residues were shown to be P59, S61, E62, T63, D65, and K67. Several of these residues were found to be charged, implicating important salt bridge interactions between the epitope and the mAbs.

Example 11 Immunohistochemistry

Tau pathology is believed to initiate within the entorhinal cortex (EC) and spread along connected neuronal pathways in the hippocampus before progressing into the cortex. To determine the reactivity of the recovered IgGs to pathogenic deposits of tau along these neuronal pathways, hippocampal tissues were obtained from an 82-year-old, non-diseased (non-AD; Abcam, Cat No. ab4305) male and an 88-year-old Alzheimer's disease (AD; Abcam, Cat. No. ab4583) male (Abcam). Cortical tissues were obtained from a 71-year-old non-diseased (non-AD) and 71-year-old Alzheimer's disease (AD) individual (Banner Sun Health). In addition to AD, there are many neurological disorders that are characterized by tau pathology, also known as tauopathies. To extend the findings, the recovered mAbs were tested in tissues obtained from progressive supranuclear palsy (PSP) and non-progressive supranuclear palsy (non-PSP) frontal lobes obtained from a 73-year-old male and an 81-year-old female, respectively (Biochain). Brain tissues were deparaffinized and rehydrated by washing twice for 10 minutes in xylene (VWR International), followed by washing twice for 3 minutes in 100% ethanol, twice for 3 minutes in 95% ethanol, twice for 3 minutes in 70% ethanol, and once for 30 seconds in distilled H2O using TISSUE-TEK® Slide Staining Set (VWR International). Tissue sections underwent heat-mediated antigen retrieval using citrate buffer (10 mM citric acid, pH 6.0) to expose antigenic sites. Sections were then incubated with blocking buffer [10% normal goat serum (Jackson ImmunoResearch, Inc.), 1% BSA and 0.3% TRITON® X-100 in PBS)] at RT for 1 hour. Excess water was removed and tissue sections were circled with an ImmEdge Hydrophobic Barrier Pen (Vector Labs). A humidified chamber was prepared by covering the bottom of a staining tray with H2O, and sections were then washed with PBS three times for 5 minutes by aspiration. Endogenous peroxidase activity was quenched in 10% H2O2 for 30 minutes at RT. Following quenching, slides were washed with PBS three times for 5 minutes by aspiration. Slides were then blocked for 1 hour at RT with a solution of 10% normal goat serum, 0.3% TRITON® X-100, 1% BSA in 1×PBS. Primary antibodies were labeled with biotin using the Zenon Human IgG Labeling Kit (Life Technologies) per manufacturer's instructions. As a negative control, a human anti-RSV-specific antibody was used. An Fc-region human-chimerized version of AT8 IgG was used as a positive control. After labeling, primary antibodies were diluted separately in blocking buffer at concentrations of 5 μg/ml and 20 μg/ml. For peptide competition experiments, 13.3 μM of cognate peptide (i.e., peptide used to recover the mAb in sorting experiments) was pre-incubated with the primary antibody for 30 minutes at RT prior to incubation with tissue sections. Tissue sections were incubated at RT for two hours with 100 μl of diluted biotin-labeled primary antibody or peptide competed antibody. After antibody was removed by aspiration, a second fixation of the tissue section was performed in 4% formaldehyde in PBS and incubated for 15 minutes at RT. The section was washed with PBS three times for 5 minutes by aspiration. Sections were then incubated for 30 minutes with streptavidin substrate VECTASTAIN® ABC Reagent (Vector Labs) before washing with PBS. Tissues were then developed with DAB substrate (Vector Labs) in the presence of nickel. Sections were then washed two times with ddH2O and allowed to completely dry at RT before mounting with 50 μl of VectaMount Permanent Mounting Medium (Vector Labs). Finally, tissue sections were counterstained with hematoxylin (Vector Labs). Representative images were acquired with Olympus BX-41 upright microscope using METAMORPH® software.

Results from the immunohistochemistry are shown in FIGS. 5A-5D. CBTAU-7.1 and CBTAU-8.1 showed positive immunoreactivity on AD brain tissues specifically, and not to healthy brain tissues, which suggests binding to pathogenic tau deposits present in diseased brain tissues. These antibodies recognize AT8-positive tau tangles and neutrophil threads in subregions of the hippocampus (FIG. 5A; entorhinal cortex) and cerebral cortex (FIG. 5B). Furthermore, the positive immunoreactivity was consistently found across multiple experiments in the neuronal cytoplasm and processes. In addition, CBTAU-18.1, 22.1, and 24.1 were also tested against hippocampal and cortical tissue sections (FIGS. 5A and 5B). Similar to CBTAU-7.1 and CBTAU-8.1, all mAbs reacted specifically to tau on AD tissue sections but not to tau on non-AD tissue sections. Of interest, CBTAU-24.1, which is not specific to phosphorylated tau, reacts specifically to diseased tau on AD tissue sections but not to tau on non-AD sections. Finally, CBTAU-16.1 and CBTAU-20.1 show reactivity to tau on both non-AD and AD tissue sections.

In addition, CBTAU-7.1, 8.1, 16.1, 18.1, 20.1, 22.1, and 24.1 were tested on cortical tissue sections corresponding to progressive supranuclear palsy (FIG. 5C). Unlike AT8, CBTAU-7.1 and CBTAU-8.1 failed to detect tau tangles in the human PSP brain, suggesting that the epitope for both mAbs is not present on PSP. CBTAU-16.1 and CBTAU-20.1 showed positive immunoreactivity to tau on non-PSP and PSP cortical brain sections, suggesting binding to both normal tau and pathogenic forms of tau. In non-AD brain sections, these antibodies showed positive immunostaining of tau in neuronal cytoplasm and processes (FIGS. 5A and 5B), yet both mAbs detected tangles and neutrophil threads in AD brain sections similar to AT8. Similar immunoreactivity as AT8 to tau tangles was also detected in PSP brain tissue sections, suggesting that both CBTAU-16.1 and CBTAU-20.1 recognize common pathogenic tau forms in other non-AD tauopathies. Furthermore, CBTAU-22.1 and CBTAU-24.1 showed immunoreactivity exclusively in AD brain tissues, with positive immunoreactivity to tangles and neutrophil threads. CBTAU-18.1 showed weak immunoreactivity in non-AD brain tissues, yet reacted stronger to AD tissue samples. CBTAU-18.1, CBTAU-22.1 and CBTAU-24.1 were also positive for tau tangles in PSP brain tissue sections (FIG. 5C).

CBTAU-27.1 and CBTAU-28.1 showed selective immunostaining in non-AD tissue sections with diffuse immunostaining in neuronal cytoplasm and processes. Interestingly, both antibodies failed to show immunoreactivity in AD tissue sections (both hippocampal and cortical), defining a novel epitope that is lost during disease progression. Unlike the majority of the human anti-tau mAbs that were identified, CBTAU-27.1 and CBTAU-28.1 were recovered by screening donor samples using an unphosphorylated peptide set spanning the entire region of human tau441. These antibodies do not require phosphorylation for binding (FIGS. 1A-11) and, as shown in FIGS. 2A-2J, do not react to PHF by ELISA. Therefore, the diffuse immunostaining pattern observed for these two mAbs was expected. In addition, CBTAU-43.1, which was originally recovered using the CBTAU-27.1 cognate peptide, was tested against cortical tissue sections. CBTAU-43.1 reacted similar to CBTAU-27.1, staining tau on non-AD but not tau on AD tissue sections. Likewise, CBTAU-46.1, 47.2 (only one variant tested), and 49.1, which were recovered using the CBTAU-28.1 cognate peptide, reacted specifically to tau on non-AD but not AD tissue sections (FIG. 5D). It is interesting to note that these mAbs all share common heavy and light chain germlines (i.e., VH5-51 and VK4-1), bind to the same regions on tau and, as shown in FIG. 5D, share similar immunohistochemical properties.

The immunohistochemistry results presented here for CBTAU-7.1, 8.1, 18.1, 22.1, 24.1, 27.1, and 28.1 have been confirmed on multiple regions of the brain and tissue samples corresponding to several non-AD and AD individuals. Immunoreactivity of CBTAU mAbs 43.1, 46.1, 47.2, and 49.1 has been confirmed once using the same tissue sample and has not yet been confirmed on samples corresponding to other AD and non-AD individuals.

Example 12 Dephosphorylation IHC

Given that the results of the IHC for CBTAU-28.1 showed immunoreactivity to tau on non-AD tissue sections but not to tau on AD tissue sections, it was hypothesized that the loss of this epitope during disease progression was a result of modification(s) (i.e., phosphorylation). To test this hypothesis, human brain tissue sections were dephosphorylated prior to assessing immunoreactivity of CBTAU-28.1. Paraffin-embedded human brain tissue sections (Abcam, cat#:ab4305, 54-year-old male, no clinical symptom vs. Abcam, cat#:ab4583, 93-year-old Hispanic female, Alzheimer disease) were deparaffinized and rehydrated by washing twice for 10 minutes in xylene (VWR International), followed by washing twice for 3 minutes in 100% ethanol, twice for 3 minutes in 95% ethanol, twice for 3 minutes in 70% ethanol, and once for 30 seconds in distilled H2O using TISSUE-TEK® Slide Staining Set (VWR International). To minimize non-specific antibody binding, tissues were never allowed to dry during washes. Tissue sections underwent heat-mediated antigen retrieval using citrate buffer (citric acid, pH 6.0) to expose antigenic sites. Excess water was removed and tissue sections were circled with an ImmEdge Hydrophobic Barrier Pen (Vector Labs). A humidified chamber was prepared by covering the bottom of a staining tray with H2O, and sections were then washed with PBS three times for 5 minutes by aspiration. Endogenous peroxidase activity was quenched in H2O2 for 15 minutes at RT. Following quenching, slides were washed with PBS three times for 5 minutes by aspiration. Sections were subsequently treated with 130 units/mL of calf intestinal alkaline phosphatase (CIAP) for 2.5 hours at 32 degrees. Slides were then blocked for 1 hour at RT with a solution of 10% normal goat serum, 0.3% TRITON® X-100, 1% BSA in 1×PBS. Murinized CBTAU-28.1 (Fc region murinized), and control mAbs AT8 and isotype control (anti-RSV mAb 4.1) were incubated overnight on hippocampal sections at a final concentration of 1 μg/mL. Sections were washed and incubated with anti-mouse, Fcγ fragment-specific antibody for 2 hours at room temperature. Samples were developed with peroxidase substrate solution DAB in the presence of Nickel. Samples were counterstained with hematoxylin (Vector Labs). Representative images were acquired with Olympus BX-41 upright microscope using METAMORPH® software.

Results are shown in FIGS. 6A and 6B. As expected, CBTAU-28.1 reacts to tau present in the non-AD hippocampal tissue sections but does not react to tau in the AD tissue sections. In contrast, control mAb, AT8, does not react to tau in non-AD sections, but clearly reacts to pathogenic tau deposits present in the AD sections (FIG. 6A). However, pretreatment of AD tissue sections with phosphatase restores reactivity of CBTAU-28.1, allowing it to stain pathogenic tau deposits present in these sections. As expected, the reactivity of AT8 was reduced with pretreatment of the AD tissue sections with phosphatase (FIG. 6B).

Example 13 Dephosphorylation ELISA

To confirm the results of Example 12, dephosphorylation of paired helical filaments was tested for reactivity to CBTAU-28.1 by ELISA. Half-area 96-well binding plates (Costar) were coated with 50 μl of antigen in TBS (2 μg/ml bovine action affinipure goat anti-human F(ab)2, and 1 μg/ml of affinity-purified paired helical filaments, iPHF, pretreated with and without calf intestinal phosphatase, CIP). Phosphatase-treated iPHF was prepared as follows. iPHF samples were resuspended in 1×NEB buffer 4 (50 mM potassium acetate, 20 mM Tris-acetate, 10 mM magnesium acetate, and 1 mM DTI) at a final concentration of 0.05 μg/ml. One unit of CIP per μg of iPHF was added (CIP, NEB Cat. No. M0290S). iPHF samples were incubated with CIP for 90 minutes at 37° C. prior to coating on ELISA binding plates. Following antigen binding overnight, the plates were washed with TBS-T and subsequently blocked with 150 μl of TBS plus 2.5% BSA for 2 hours at RT. Purified control and anti-tau IgG, CBTAU-28.1), were titrated in five-fold dilutions starting at 25 μg/ml in TBS/0.25% BSA, and IgGs and incubated for 1.5 hours. Plates were washed four times with TBS-T and secondary antibody (anti-human Fab HRP, Jackson Immunoresearch, Cat. No. 109-036-097) was added and incubated at RT for 45 minutes. Following incubation, plates were washed four times in TBS-T and developed with SureBlue Reserve TMB Microwell Peroxidase Substrate (KPL) for approximately 2 minutes. The reaction was immediately halted by the addition of TMB Stop Solution (KPL) and the absorbance at 450 nm was measured using an ELISA plate reader. Each experimental point was performed in triplicate.

Results are shown in FIG. 7. As previously shown in Example 7, CBTAU-28.1 reacts poorly to iPHF by ELISA in contrast to AT8. However, dephosphorylation of iPHF with CIP restores the reactivity of CBTAU-28.1 to the filamentous sample. As expected, the reactivity of the phospho-tau control mAb, AT8, is abolished after dephosphorylation of iPHF with CIP.

Example 14 Reactivity of CBTAU-27.1, 28.1, 43.1, 47.1, 47.2 and 49.1 to Phosphopeptides

The immunohistochemical results for CBTAU-27.1 (and CBTAU-43.1) and CBTAU-28.1 (and CBTAU-46.1, 47.2, 49.1) suggest that these mAbs react with an epitope on tau that is present in normal, non-AD, tissue sections but is lost or masked during the disease setting (FIGS. 5A-5D). It was hypothesized that this was a result of a phosphorylation event within the region that results in masking of the epitope(s). The experiments highlighted in Examples 12 and 13 showed that this was indeed true for 28.1. Therefore, it was desired to specifically identify the site(s) that could potentially be targeted for phosphorylation and account for loss of reactivity for CBTAU-28.1. Because 47.1, 47.2, and 49.1 bound to the same region on tau as CBTAU-28.1 (i.e., 52-71), it was decided to test these mAbs as well in these experiments. In addition, the same exercise was carried out for CBTAU-43.1 and CBTAU-27.1 as they behave similarly to CBTAU-28.1 by IHC.

Singly and dually phosphorylated-tau peptides were designed to cover all potential phosphorylation sites with regions 52-71 and 299-323 (CBTAU-28.1 and CBTAU-27.1 binding region, respectively). CBTAU-27.1 and CBTAU-43.1 mAbs were tested against the peptides listed on Tables 30 and 32. 96-well streptavidin-coated ELISA plates (Pierce) were coated with phosphorylated tau peptides as detailed in Example 9. Purified anti-tau IgGs were diluted to 5 μg/ml in TBS containing 0.25% BSA, and titrated five-fold. Antibody control and secondary antibodies were used as detailed in Example 9. Antibody reactivity at 1 μg/mL was determined by ELISA and scored as no binding (−), weak (−/+), moderate (+), or strong (++). (−) for average of two O.D. 450 nm readings <0.3; (−/+) for >0.5 and <1.0; (+) for >1.0 and <1.5; (++) for >1.5. Results for each antibody are shown in Tables 30-34 and FIGS. 8A-8F.

TABLE 30 CBTAU-27.1: Peptides for reactivity by ELISA SEQ ID Peptide NO Result tau 299-369 331 HVPGGGSVQIVYKPVDLSKVTSKCGSLG ++ NIHHKPGGGQVEVKSEKLDFKDRVQSKI GSLDNITHVPGGGNK tau 299-323 458 HVPGGGSVQIVYKPVDLSKVTSKCG ++ ptau 299-323 503 HVPGGG(pS)VQIVYKPVDLSKVTSKCG ++ p305 ptau 299-323 504 HVPGGGSVQIV(pY)KPVDLSKVTSKCG ++ p310 ptau 299-323 505 HVPGGGSVQIVYKPVDL(pS)KVTSKCG − p316 ptau 299-323 506 HVPGGGSVQIVYKPVDLSKV(pT)SKCG ++ p319 ptau 299-323 507 HVPGGGSVQIVYKPVDLSKVT(pS)KCG ++ p320 ptau 299-323 508 HVPGGG(pS)VQIV(pY)KPVDLSKVTS ++ p305, 310 KCG ptau 299-323 509 HVPGGG(pS)VQIVYKPVDL(pS)KVTS − p305, 316 KCG ptau 299-323 510 HVPGGG(pS)VQIVYKPVDLSKV(pT)S ++ p305, 320 KCG ptau 299-323 511 HVPGGG(pS)VQIVYKPVDLSKVT(pS) ++ p305, 321 KCG ptau 299-323 512 HVPGGGSVQIV(pY)KPVDL(pS)KVTS − p310, 316 KCG ptau 299-323 513 HVPGGGSVQIV(pY)KPVDLSKV(pT)S ++ p310, 320 KCG ptau 299-323 514 HVPGGGSVQIV(pY)KPVDLSKVT(pS) ++ p310, 321 KCG ptau 299-323 515 HVPGGGSVQIVYKPVDL(pS)KV(pT)S − p316, 320 KCG ptau 299-323 516 HVPGGGSVQIVYKPVDL(pS)KVT(pS) − p316, 321 KCG ptau 299-323 517 HVPGGGSVQIVYKPVDLSKV(pT)(pS) −/+ p320, 321 KCG

TABLE 31 CBTAU-28.1: Peptides for reactivity by ELISA SEQ ID Peptide NO. Result tau 42-103 325 GLKESPLQTPTEDGSEEPGSETSDAKS ++ TPTAEDVTAPLVDEGAPGKQAAAQPHT EIPEGTTA tau 48-71 518 LQTPTEDGSEEPGSETSDAKSTPT ++ ptau 48-71 519 LQTPTEDGSEEPGSETSDAKSTP(pT) ++ (p71) ptau 48-71 520 LQTPTEDGSEEPGSE(pT)SDAKSTPT − (p63) ptau 48-71 521 LQTPTEDGSEEPG(pS)ETSDAKSTPT − (p61) ptau 48-71 522 LQTPTEDG(pS)EEPGSETSDAKSTPT ++ (p56) ptau 48-71 523 LQTP(pT)EDGSEEPGSETSDAKSTPT ++ (p52) ptau 48-71 524 LQTPTEDGSEEPGSETSDAK(pS)TPT ++ (p68) ptau 48-71 525 LQTPTEDGSEEPGSETSDAKS(pT)PT ++ (p69) ptau 48-71 526 LQTPTEDGSEEPGSET(pS)DAKSTPT ++ (p64) ptau 48-71 527 LQTPTEDGSEEPG(pS)ET(pS)DAKS − (p61, p64) TPT ptau 48-71 528 LQTPTEDGSEEPG(pS)E(pT)SDAKS − (p61, p63) TPT ptau 48-71 529 LQTPTEDGSEEPGSE(pT)(pS)DAKS − (p63, p64) TPT

TABLE 32 CBTAU-43.1: Peptides for reactivity by ELISA SEQ ID Peptide NO. Result tau 299-369 331 HVPGGGSVQIVYKPVDLSKVTSKCGSLG ++ NIHHKPGGGQVEVKSEKIDFKDRVQSKI GSLDNITHVPGGGNK tau 299-323 458 HVPGGGSVQIVYKPVDLSKVTSKCG ++ ptau 299-323 503 HVPGGG(pS)VQIVYKPVDLSKVTSKCG ++ p305 ptau 299-323 504 HVPGGGSVQIV(pY)KPVDLSKVTSKCG ++ p310 ptau 299-323 505 HVPGGGSVQIVYKPVDL(pS)KVTSKCG − p316 ptau 299-323 506 HVPGGGSVQIVYKPVDLSKV(pT)SKCG ++ p319 ptau 299-323 507 HVPGGGSVQIVYKPVDLSKVT(pS)KCG ++ p320 ptau 299-323 508 HVPGGG(pS)VQIV(pY)KPVDLSKVTS ++ p305, 310 KCG ptau 299-323 509 HVPGGG(pS)VQIVYKPVDL(pS)KVTS − p305, 316 KCG ptau 299-323 510 HVPGGG(pS)VQIVYKPVDLSKV(pT)S ++ p305, 320 KCG ptau 299-323 511 HVPGGG(pS)VQIVYKPVDLSKVT(pS) ++ p305, 321 KCG ptau 299-323 512 HVPGGGSVQIV(pY)KPVDL(pS)KVTS − p310, 316 KCG ptau 299-323 513 HVPGGGSVQIV(pY)KPVDLSKV(pT)S ++ p310, 320 KCG ptau 299-323 514 HVPGGGSVQIV(pY)KPVDLSKVT(pS) ++ p310, 321 KCG ptau 299-323 515 HVPGGGSVQIVYKPVDL(pS)KV(pT)S −/+ p316, 320 KCG ptau 299-323 516 HVPGGGSVQIVYKPVDL(pS)KVT(pS) − p316, 321 KCG ptau 299-323 517 HVPGGGSVQIVYKPVDLSKV(pT)(pS) ++ p320, 321 KCG

TABLE 33 CBTAU-47.1 and CBTAU-47.2: Peptides for reactivity by ELISA SEQ Result Result ID CBTAU- CBTAU- Peptide NO. 47.1 47.2 tau 325 GLKESPLQIPTEDGSEEPGSETSD ++ ++ 42- AKSIPTAEDVTAPLVDEGAPGKQA 103 AAQPHTIPEGTTA tau 518 LQTPTEDGSEEPGSETSDAKSTPT ++ ++ 48- 71 ptau 519 LQTPTEDGSEEPGSETSDAKSTP ++ ++ 48- (pT) 71 (p71) ptau 520 LQTPTEDGSEEPGSE(pT)SDAK − − 48- STPT 71 (p63) ptau 521 LQTPTEDGSEEPG(pS)ETSDAK − − 48- STPT 71 (p61) ptau 522 LQTPTEDG(pS)EEPGSETSDAK ++ ++ 48- STPT 71 (p56) ptau 523 LQTP(pT)EDGSEEPGSETSDAK ++ ++ 48- STPT 71 (p52) ptau 524 LQTPTEDGSEEPGSETSDAK(pS) ++ ++ 48- TPT 71 (p68) ptau 525 LQTPTEDGSEEPGSETSDAK(pT) ++ ++ 48- PT 71 (p69) ptau 526 LATPTEDGSEEPGSET(pS)DAK ++ ++ 48- STPT 71 (Ser64) ptau 527 LQTPTEDGSEEPG(pS)ET(pS) − − 48- DAKSTPT 71 (p61, Ser64) ptau 528 LQTPTEDGSEEPG(pS)E(pT) − − 48- SDAKSTPT 71 (p61, p63) ptau 529 LQTPTEDGSEEPGSE(pT)(pT) − − 48- (pS)DAKSTPT 71 (p63, p64)

TABLE 34 CBTAU-49.1: Peptides for reactivity by ELISA SEQ ID Peptide NO. Result tau 325 GLKESPLQTPTEDGSEEPGSETSDAKSTPTA ++ 42- EDVTAPLVDEGAPGKQAAAQPHTEIPEGTTA 103 tau 518 LQTPTEDGSEEPGSETSDAKSTPT ++ 48-71 ptau 519 LQTPTEDGSEEPGSETSDAKSTP(pT) ++ 48-71 (p71) ptau 520 LQTPTEDGSEEPGSE(pT)SDAKSTPT − 48-71 (p63) ptau 521 LQTPTEDGSEEPG(pS)ETSDAKSTPT − 48-71 (p61) ptau 522 LQTPTEDG(pS)EEPGSETSDAKSTPT ++ 48-71 (p56) ptau 523 LQTP(pT)EDGSEEPGSETSDAKSTPT ++ 48-71 (p52) ptau 524 LQTPTEDGSEEPGSETSDAK(pS)TPT ++ 48-71 (p68) ptau 525 LQTPTEDGSEEPGSETSDAKS(pT)PT −/+ 48-71 (p69) ptau 526 LQTPTEDGSEEPGSET(pS)DAKSTPT ++ 48-71 (Ser64) ptau 527 LQTPTEDGSEEPG(pS)ET(pS)DAKSTPT − 48-71 (p61, Ser64) ptau 528 LQTPTEDGSEEPG(pS)E(pT)SDAKSTPT − 48-71 (p61, p63) ptau 529 LQTPTEDGSEEPGSE(pT)(pS)DAKSTPT − 48-71 (p63, p64)

The results for CBTAU-27.1 and CBTAU-43.1 show that phosphorylation at S316 is sufficient to completely inhibit reactivity (Table 30 and Table 32). This suggests that the loss in reactivity to tau on AD tissue sections (Example 11) may be due to phosphorylation at S316, an event that may occur early during the course of the disease. For CBTAU-28.1, 47.1, 47.2, 49.1, phosphorylation at either S61 or T63 is sufficient to completely inhibit reactivity. Taken together, the results for CBTAU-28.1, 47.1, 47.2, and 49.1 suggest that phosphorylation at S61 and/or T63 is a mechanism that accounts for loss of this epitope during the course of the disease.

Example 15 Generation of Anti-Tau mAb Mouse-Human Chimeras and Human Isotypes

To test the efficacy of the human anti-tau mAbs in a mouse model of tauopathy, mouse-human antibody chimeras were generated by replacing the human Fc region with a mouse IgG1 Fc. Briefly, the human IgG1 CH1 region was amplified from the pCB-IgG vector using primers Step1HMchim-Fwd and Step1HMchim-Rev (Table 35) to generate a 0.95 kb fragment containing a 5′-XhoI site (frag. 1). Mouse IgG1 CH2 and CH3 domains (Fc region) are amplified from a gene-synthesized construct using primers Step2HMchim-Fwd and Step2HMchim-Rev (Table 30) to generate a 0.82 kb fragment (frag. 2). A third fragment (frag. 3) was generated by amplifying the polyA region of the pCB-IgG vector using primers Step3HMchim-Fwd and Step3HMchim-Rev (Table 30), which includes a 3′-DraIII site. The three fragments were linked into a single cassette by overlap extension PCR to generate a 2.3 kb overlap fragment harboring the human CH1 followed by the mouse CH2-CH3 domains. The overlap fragment was subsequently cloned via the XhoI and DraIII sites into the pCB-IgG CBTAU-7.1 vector to generate a mouse-human chimera of CBTAU-7.1, containing the human variable, CH1, hinge and Ck regions followed by the mouse CH2 and CH3 regions. CBTAU-22.1, 24.1, 27.1, 28.1, 47.1, 47.2, 46.1, 49.1, and 43.1 chimeras were then generated by digesting the CBTAU-7.1 chimera construct and pCB-IgG CBTAU human mAb constructs with XhoI and XbaI, and the corresponding fragments were subcloned. Nucleotide sequences for all constructs are verified according to standard techniques known to the skilled artisan. Chimeric antibodies were subsequently expressed and purified as detailed in Example 5 using Protein G agarose instead of Protein A.

TABLE 35 Primers For Mouse-Human Chimerization SEQ ID Primer ID DNA SEQUENCE (5′-3′) NO: Step1HMchim- TCTCCGCCGGTGAGTCTCGAGGC 530 Fwd Step1HMchim- TGTCCCTGGATGCAGGCTACTCTAGG 531 Rev Step2HMchim- AGAGTAGCCTGCATCCAGGGACAG 532 Fwd Step2HMchim- TCTAGATCATTTACCAGGAGAGTGGG AGAG 533 Rev Step3HMchim- TCTCCTGGTAAATGATCTAGAGTTTAAACCGCTG 534 Fwd Step3HMchim- ATGGCCCACTACGTGAACCATCACC 535 Rev

Example 16 Preparation of IgG2, 3 and 4 Isotypes

As mentioned in Example 3, all CBTAU mAbs were cloned and expressed as chimeric human IgG1 regardless of their native isotype. To generate additional human isotype versions (i.e., IgG2/3/4), the CH1 through CH3 region corresponding to each of the human IgG isotypes is PCR amplified from gene-synthesized constructs containing the corresponding constant regions, hinge, and intron sequences. The PCR amplicons contain 5′-XhoI and 3′-DraIII sites, which are used to subclone the fragments into the corresponding pCB-IgG CBTAU antibody construct. In this manner, human IgG2, 3 and 4 isotype versions are generated for each of the anti-tau mAbs.

Example 17 Generation of De-Risked and Fc-Engineered Anti-Tau Chimeric Monoclonal Antibody Variants

The heavy and light chain variable regions (VH and VL) for each anti-tau antibody clone isolated in Example 3 are analyzed for the presence of free cysteines and potential post-translational modification sites, which include glycosylation, deamidation and oxidation sites. Amino acid mutations consisting of structurally conserved and/or germline-based substitutions are used to change these sites. Non-conserved cysteines in the variable regions are mutated to serine. For glycosylation sites, several mutations are used, including replacement of asparagine for the conservative glutamine or germline mutations. Modifications to the deamidation sites include replacement of aspartic acid for asparagine and serine or alanine for glycine. Sites of potential oxidation are not modified. To increase the binding affinity to FcRn and thus increase the half-life of IgG1 mAbs in vivo, several mutations located at the boundary between the CH2 and CH3 regions are generated. These mutations included M252Y/S254T/T256E plus H433K/N434F (C. Vaccaro et al., 2005) or T250Q/M428L (P. R. Hinton et al., 2004), which have been shown to increase IgG1 binding to FcRn. All substitutions are generated by site-directed mutagenesis per manufacturer's instructions (QUICKCHANGE™ II, Agilent Technologies, cat. no. 200521). Nucleotide sequences for all constructs are verified according to standard techniques known to the skilled artisan. 

What is claimed is:
 1. A method for the prophylaxis and/or treatment of a subject for Alzheimer's disease, or the memory and/or cognitive disorders associated with tau, the method comprising: utilizing an antibody or an antigen-binding fragment thereof in the prophylaxis and/or treatment of Alzheimer's disease, or memory and/or cognitive disorders associated with tau in a subject, wherein the antibody is selected from the group consisting of a) an antibody comprising a heavy chain CDR1 region of SEQ ID NO:201, a heavy chain CDR2 region comprising SEQ ID NO:202, and a heavy chain CDR3 region comprising SEQ ID NO:203, a light chain CDR1 region comprising SEQ ID NO:204, a light chain CDR2 region comprising SEQ ID NO:205 and a light chain CDR3 region comprising SEQ ID NO:206, b) an antibody comprising a heavy chain CDR1 region comprising SEQ ID NO:207, a heavy chain CDR2 region comprising SEQ ID NO:208, and a heavy chain CDR3 region comprising SEQ ID NO:209, a light chain CDR1 region comprising SEQ ID NO:210, a light chain CDR2 region comprising SEQ ID NO:211 and a light chain CDR3 region comprising SEQ ID NO:212, c) an antibody comprising a heavy chain CDR1 region comprising SEQ ID NO:222, a heavy chain CDR2 region comprising SEQ ID NO:223, and a heavy chain CDR3 region comprising SEQ ID NO:224, a light chain CDR1 region comprising SEQ ID NO:225, a light chain CDR2 region comprising SEQ ID NO:173 and a light chain CDR3 region comprising SEQ ID NO:226; d) an antibody comprising a heavy chain CDR1 region comprising SEQ ID NO:238, a heavy chain CDR2 region comprising SEQ ID NO: 239, and a heavy chain CDR3 region comprising SEQ ID NO:240, a light chain CDR1 region comprising SEQ ID NO:241, a light chain CDR2 region comprising SEQ ID NO:173 and a light chain CDR3 region comprising SEQ ID NO:242, e) an antibody comprising a heavy chain CDR1 region comprising SEQ ID NO:243, a heavy chain CDR2 region comprising SEQ ID NO:244, and a heavy chain CDR3 region comprising SEQ ID NO:245, a light chain CDR1 region comprising SEQ ID NO:246, a light chain CDR2 region comprising SEQ ID NO: 173 and a light chain CDR3 region comprising SEQ ID NO:212, f) an antibody comprising a heavy chain CDR1 region comprising SEQ ID NO:243, a heavy chain CDR2 region comprising SEQ ID NO:247, and a heavy chain CDR3 region comprising SEQ ID NO:248, a light chain CDR1 region comprising SEQ ID NO:249, a light chain CDR2 region comprising SEQ ID NO:173 and a light chain CDR3 region comprising SEQ ID NO:212, and g) an antibody comprising a heavy chain CDR1 region comprising SEQ ID NO:250, a heavy chain CDR2 region comprising SEQ ID NO:251, and a heavy chain CDR3 region comprising SEQ ID NO:252, a light chain CDR1 region comprising SEQ ID NO:254, a light chain CDR2 region comprising SEQ ID NO:254 and a light chain CDR3 region comprising SEQ ID NO:255.
 2. A method for detecting or diagnosing Alzheimer's disease, or memory and/or cognitive disorders associated with tau in a human subject, the method comprising: assaying the level of tau antigen in a biological sample taken from the subject utilizing the antibody of claim 1 or an antigen-binding fragment thereof.
 3. The method of according to claim 2, wherein the biological sample comprises peripheral blood, serum, plasma, urine, cerebrospinal fluid, tissue biopsy, surgical specimen, fine needle, aspirates, autopsy material, cell culture supernatant, isolated cells, fermentation supernatant, or tissue homogenate. 